Energy & Fuels 1990,4,675-688

Preparation of Bacteriopetroporphyrins by Partial Synthesis from the Chlorobium Chlorophylls

Norman W. Smith and Kevin M. Smith* Department of Chemistry, University of California, Davis, California 95616

Received April 27, 1990. Revised Manuscript Received July 12, 1990

675

Chemical degradation of the natural bacteriochlorophyll d homologous mixture to give the cor- responding bacteriopetroporphyrin methyl esters is described. Reduction of the corresponding methyl bacteriopheophorbide d homologue with excess of sodium borohydride, followed by oxidation with 2,3-dichloro-5,6-dicyanobenzoquinone, affords the corresponding bacteriopetroporphyrin. 'H NMR spectroscopy of the nickel(I1) complexes is used to establish that the pigments are identical with those isolated from immature Messel oil shale. Similar degradative transformations of the bacteriochlorophyll c homologues (and also of the bacteriochlorophyll e mixture) to give "bacteriopetroporphyrins C" (which have not yet been observed in oil shales) are reported, and the proton NMR signatures of their nickel(I1) complexes are obtained and assigned.

Introduction Alfred Treibs was the first to discover petroporphyrins

in petroleum oil shales, coals, etc. In the 1 9 3 0 ~ , ~ ~ ~ he iso- lated and identified the major metalloporphyrin present in petroleum sources, vanadyl deoxophylloerythroetio- porphyrin (DPEP) (1) and vanadyl etioporphyrin 111. In

2b CH,

1

1936 it was proposed3 that these compounds were degra- dation products of the chlorophylls and hemins and a scheme was suggested to account for their origin. New petroporphyrins continue to be isolated and identified, and it has recently been stated4 that there are now over 40 confirmed structures. The petroporphyrins are now gen- erally accepted to be derived by geochemical degradation of chlorophyll over and there is significant recent evidence in support of

There has been much speculation about the origin of petroporphyrins containing more than 32 carbons. One possible source for higher molecular weight petroporphy- rins would be the Chlorobium chlorophylls (such as the bacteriochlorophylls c , d , and e , which have homologated side chains at positions 4 and 5 and, for the bacterio- chlorophylls c and e, also at the &meso position). However, early analyses of maleimides from degradation of high molecular weight geoporphyrins showed that not only is

(1) Treibs, A. Liebigs Ann. Chem. 1934, 510, 42. (2) Treibs, A. Liebigs Ann. Chem. 1934, 509, 103. (3) Treibs, A. Angew. Chem. 1936,49,682. (4) See other papers in this issue of Energy Fuels. (5) Quirke, J. M. E.; Eglinton, G.; Maxwell, J. R. J . Am. Chem. SOC.

(6) Quirke, J. M. E.; Maxwell, J. R. Tetrahedron 1980,36, 3453. (7) Quirke, J. M. E.; Maxwell, J. R.; Eglington, G.; Sanders, J. K. M.

(8) Fookes, C. J. R. J. Chem. Soc., Chem. Commun. 1983, 1472. (9) Fookes, C. J. R. J . Chem. SOC., Chem. Commun. 1983, 1474. (10) Verne-Mismer, J.; Ocampo, R.; Callot, H. J.; Albrecht, P. Tetra-

(11) Fookes, C. J. R. J . Chem. SOC., Chem. Commun. 1985, 706.

1970, 101, 7693.

Tetrahedron Lett . 1980,21, 2897.

hedron Lett . 1986,27, 5257.

the 4-isobutyl substituent on pyrrole subunit B not f o ~ n d , ~ ~ - l ~ but Quirke and co-~orkers '~ found alkyl sub- stituents containing up to 11 carbons that could not have arisen from simple degradation of Chlorobium chloro- phylls. This led Baker and PalmerI2 to conclude that the likelihood of the Chlorobium chlorophylls being precursors to certain petroporphyrins was small because trans- alkylation mechanisms can satisfactorily explain higher molecular weight porphyrins.

Recently, however, Ocampo and colleague^^^^^ have isolated a series of petroporphyrins from Messel oil shale that have homologous side chains a t positions 4 and 5 showing a clear origin from photosynthetic (Chlorobium) bacteria. In a preliminary publication, we have reported their syntheses.18 Thus it is apparent that while the Chlorobium-type chlorophylls are contributors to the wide variety of petroporphyrins, they are probably not a major source for higher molecular weight porphyrins found in mature sediments or petr01eum.l~

Results and Discussion Although there are over 70 known petr~porphyrins,~

many of them have been structurally characterized only by NMR [with appropriate 2D and nuclear Overhauser enhancement (NOE) studies]. Although this method is an excellent characterization technique, for an organic chemist the ultimate proof of structure is total or partial synthesis using rational synthetic approaches; it is always reassuring to verify the NMR data by conducting a syn- thesis of the molecule in question and then comparing the data for the synthetic material against that of the natural product.

(12) Baker, E. W.; Palmer, S. E. In The Porphyrins; Dolphin, D., Ed.; Academic Press, New York, 1978; Vol. 1, pp 486-552.

(13) Quirke, J. M. E.; Shaw, G. J.; Soper, P. D.; Maxwell, J. R. Tet- rahedron 1980, 36, 3621.

(14) Barwise, A. J. G.; Whitehead, E. V. In Adoances in Organic Geochemistry; Maxwell, J. R., Douglas, A. G., Eds.; Pergamon Press: Oxford, 1980; pp 181-92.

(15) Ocampo, R.; Callot, H. J.; Albrecht, P. J . Chem. Soc., Chem. Commun. 1985, 198.

(16) Ocampo, R.; Callot, H. J.; Albrecht, P. J . Chem. Soc., Chem. Commun. 1985, 200.

(17) Ocampo, R.; Callot, H.; Albrecht, P. In Metal Complexes in Fossil Fuels; Filby, R. H., Branthaver, J. F., Eds.; American Chemical Society: Washington, DC, 1987; pp 68-72.

(18) Smith, N. W.; Smith, K. M. J. Chem. SOC., Perkin Trans. 1 1989, 188.

(19) Filby, R. H.; Van Berkel, G. In Metal Complexes in Fossil Fuels; Filby, R. H., Branthaver, J. F., Eds.; American Chemical Society: Washington, DC, 1987; pp 2-39.

0887-0624/90/2504-0675$02.50/0 0 1990 American Chemical Society

676 Energy & Fuels, Val. 4, No. 6, 1990

Chart I. Structures of Bacteriopetroporphyrins Isolated from Messel Oil Shale (as Methyl Esters) and

Characterized by Ocampo et al.16

Smith and Smith

Chart 11. Structures of Bacteriochlorophyll d Homologues (2) and of Corresponding Methyl Bacteriopheophorbides d

(4)

I " I CO*CH,

3

R4 RS R4 RS

Total synthesis (especially of an unsymmetrical por- phyrin) requires a large number of steps and therefore requires much time and effort in order to carry through the procedure. On the other hand, performing a partial synthesis can greatly simplify matters depending on the starting material, target molecule, and the routes available to achieve conversion. In the present case, the petropor- phyrins that were recently discovered in Messel oil shale by Ocampo et (Chart I) were a particularly convenient system to study because of the readily available bacter- iochlorophylls d (Chart 11) to which those particular pet- roporphyrins are so clearly related. In a certain sense, conversion of the bacteriochlorophylls d into the corre- sponding Messel oil bacteriopetroporphyrins would con- stitute a biomimetic synthesis. The skeletal relationship between structures %a,e,f,g and 3a-d is clear. The methyl bacteriopheophorbides d (Bmph-d) (4) are readily obtained from the bacteriochlorophylls d, and the steps necessary to achieve the desired conversion of pheophorbides into the required porphyrins were envisioned to be possible, so the partial syntheses described below were undertaken.

The green and brown sulfur bacteria are found in stagnant ponds, lakes, and estuarine habitats having vertical gradients of light (from above) and hydrogen sulfide (from be lo^).^ The main light-harvesting antenna of these sulfur bacteria are the homologous series of bac- teriochlorophylls c, d, and e known as the Chlorobium chlorophylls.21 The bacteriochlorophylls d were first isolated from Chlorobium thiosulfatophilum and identified by Holtn-24 and MacDonald and co-workers.25 The main esterifying alcohol a t the 7-propionic position was deter- mined to be farnesol.21 Smith and co-workers subsequently verified the stereochemistry of the 2-(l-hydroxyethyl) group for the homologues by NMR, HPLC, and X-ray analysis.26

For the bacteriochlorophylls d, cultures of Chlorobium vibrioforme forma thiosulfatophilum were grown on the

(20) Simpson, D. J.; Smith, K. M. J. Am. Chem. SOC. 1988,110,1753. (21) Holt, A. S. In The Chlorophylls; Vernon, L. P., Seely, G. R., Eds.;

(22) Holt, A. S.; Purdie, J. W. Can. J. Chem. 1965, 43, 3347. (23) Holt, A. S.; Hughes, D. W. J. Am. Chem. SOC. 1961, 83, 499. (24) Holt, A. S.; Hughes, D. W.; Kende, H. J.; Purdie, J. W. J. Am.

(25) Archibald, J. L.; Walker, D. M.; Shaw, K. B.; Markovac, A.;

(26) Smith, K. M.; Goff, D. A. J. Chem. Soc., Perkin Trans. I 1985,

Academic Press: New York, 1966; p 111.

Chem. SOC. 1962,84, 2835.

MacDonald, S. F. Can. J . Chem. 1966,44, 345.

1099.

2 M = Mg, R = Famesyl (Bacteriochlorophylls-d)

4 M = 2H, R = Methyl (Methyl Bacteriopheophorbides-d)

4.5- or 20-L scale for several days as described elsewhere.% The cells were collected by centrifugation and extracted with methanol, and a crude mixture of carotenoids and bacteriochlorophylls d was obtained. Treatment of the extract with sulfuric acid in methanol served to demetalate and transesterify the 7-propionic ester to give the ho- mologous series of Bmph-d (4). The 5-ethyl series of ho- mologues was separated from the 5-methyl series by preparative normal-phase HPLC, and the homologues within each subset were then separated by preparative reverse-phase HPLC.

On paper, the necessary steps to achieve conversion of the Bmph-d (4) to the desired petroporphyrins 3 included (i) reduction of the 2-hydroxyethyl group to ethyl, (ii) reduction of the 9-keto to methylene, and (iii) oxidation of the chlorin to the porphyrin macrocycle. The porphyrin could then be chelated with nickel for proton NMR in- vestigation. Procedures chosen to accomplish these steps had to leave the 7-methyl propionate substituent intact (Le., no reduction). Initial considerations included the following: Removal of the hydroxy group from the 2- hydroxyethyl substituent is fairly straightforward. Deh- ydration of hydroxyethyl groups by treatment with a catalytic amount of p-toluenesulfonic acid in hot 1,2-di- chlorobenzenez7 has been done before on porphyrin com- pounds. This could then be followed by catalytic hydro- genation of the resulting vinyl group to give the ethyl group. Oxidations of chlorins to porphyrins can be effected by treatment with high potential quinones such as 2,3- dichloro-5,6-dicyano-1,4-benzoquinone (DDQ).28 Atten- tion, therefore, was focused first to determining an efficient way of removing the 9-keto group.

Baker et al.29 reported that treatment of pheophytins with hydrazine hydrate and strong base in triethylene glycol a t high temperature (Wolff-Kishner conditions) effected reduction of the 9-keto group to methylene and also accomplished oxidation of the chlorin to the corre-

~~~~-

(27) Smith, K. M. Porphyrins and Metalloporphyrins; Smith, K. M . ,

(28) Kenner, G. W.; McCombie, S. W.; Smith, K. M. J. Chem. Soc.,

(29) Baker, E. W.; Corwin, A. H.; Klesper, E.; Wei, P. E. J. Org. Chem.

Ed.; Elsevier: Amsterdam, 1975.

Perkrn Trans. 1 1973, 2517.

1968,33,3144.

Preparation of Bacteriopetroporphyrins

Scheme I. Wolff-Kischner Degradation of Bmph-d

M e M R 4

Energy & Fuels, Vol. 4, No. 6, 1990 677

Scheme I1 Et Me Et Me

7 +

13% C0,Me

sponding porphyrin. When [n-Pr,Et]-Bmph-d (4f) was subjected to the same conditions, the desired compound was obtained, but in rather disappointing yields. Only 13% of the porphyrin and 4% of the corresponding chlorin were obtained (Scheme I).

Since reduction of the 9-keto group can readily be ac- complished with NaBH, in virtually quantitative yield, methods for conversion of the 9-keto group into the cor- responding hydroxy group, followed by reductive deoxy- genation, were next investigated. Also at this point, it was decided to try model reductive studies on methyl meso- pyropheophorbide a (5), because of its more ready avail- ability (compared with Bmph-d) from Spirulina maxima alga.

Although reduction of aliphatic alcohols can seldom be accomplished by hydrogenolysis,3° reduction of benzylic- type alcohols can often be performed in this way. Tech- niques to accomplish this objective have been reviewed by R ~ l a n d e r . ~ ~ As a model system, 5 was reduced to the 9-hydroxy compound 6 with NaBH, and then this was hydrogenated over 10% palladized charcoal in an attempt to obtain the 9-deoxo compound 7; however, only starting

&NH N3 Me," ' W M e

R2

A R ' Me02C

5 R',' = 0 6 R' = H, R2 = OH 7 R ' ' = H

material 6 was recovered. The attempted hydrogenation of the same compound in the presence of trifluoroacetic acid (TFA)32 was also unsuccessful, this causing decom- position of the starting material. Attempts to deoxygenate with P21t3 or with triethylsilane in the presence of TFA% gave very small amounts of product as determined by thin-layer chromatography (TLC).

Raney nickel has been used to reduce nickel(I1) com- plexes of methyl pyropheophorbide a to provide mixtures

(30) March, J. Advanced Organic Chemistry; Wiley: New York, 1985. (31) Rylander, P. N. Catalytic Hydroaenation over Platinum Metals: - -

Academic Press:. New York,-1967. (32) Dar'eva; Miklukhin, J. Gen. Chem. USSR 1959,29, 620. (33) Suzuki, H.; Tani, H.; Kubota, H.; Sato, N. Chem. Lett. 1983,247. (34) Adlington, M. G.; Orfanopoulos, M.; Fry, J. L. Tetrahedron Lett.

1976, 2955.

Me' ' W M e Me" " W M e

ti CHO CHO H -

I Me0,C

a Me0,C

9

of its corresponding 9-deoxo compound and di-, tetra-, and hexahydr~porphyrins.~~~~ Although the conditions have been worked out to give the 9-deoxo compound 7 in yields as high as 52%, similar treatment of Bmph-d (4) gave a mixture of several compounds, all in disappointingly minor amounts.

An attempt to dehydrate the 9-hydroxy group of 6 by acid catalysis to give the 9,lO-dehydro compound followed by catalytic hydrogenation gave similar results as obtained previou~ly .~~ The product isolated was identified as a 9,lO-diformylchlorin. Apparently the dehydration pro- ceeds to give the exocyclic alkeno ring 8 which is then attacked by dioxygen in air to give the ring-opened com- pound 9 (Scheme 11).

Other methods to accomplish these reductive deoxy- genations are abundant; they include the Clemmensen

hydride reagents in combination with Lewis acids such as LiA1H4/A1C13,39s40 and many others.30 Less direct methods, such as conversion of the hydroxy group to the tosylate or another sulfonate ester, followed by displacement with LiA1H4,41-43 with NaBH, in a dipolar aprotic solvent,44 with LiEt3BH, and with Bu3SnH-Na16 are also available. Use of LiAlH, was not an option in our case, however, because that would have also reduced the propionic ester.

The following method proved to be quite successful. It is a modification of work developed earlier involving the use of hydrides in conjunction with Lewis acids. Gribble and co-workersa reported that reduction of aryl carbonyl and hydroxy groups proceeded in high yield upon treat- ment with NaBH, in the presence of TFA. This method seemed particularly well suited for use on the Bmph since they contain both aryl alcohol and aryl ketone function- alities. I t was hoped that this NaBH,/TFA method could provide both reduction of the 2-hydroxyethyl to ethyl and also of the 9-keto to 9-CH2. Model studies using methyl pyropheophorbide a ( 5 ) gave encouraging results (75% yield of 7), so it was applied to the Bmph-d. Small-scale treatment of the homologous mixture 4e-h also gave very encouraging results, so conversion of a single homologue into its corresponding deoxo compound was attempted next.

Because Ocampo et al.16 reported full NOE data for the

Goff, D. A. Ph.D. Dissertation, University of California, Davis,

Mengler, C.-D. Dissertation, Braunschweig, 1966. Lai, J.-J. PbD. Diasertation, University of Califomia, Davis, 1983. Martin, E. L. Org. React. 1942, 1 , 155. Brown, H. C.; Subba Rao, B. C. J. Am. Chem. SOC. 1956,78,2582. Blackwell, J.; Hickinbottom, W. J. J. Chem. SOC. 1961, 1405. Dimitriadis. E.: Massy-Westrop. R. A. Aust. J. Chem. 1982.35.

1895. (42) Eschenmoser, A.; Frey, A. Helv. Chim. Acta 1952, 35, 1660. (43) Rapoport, H.; Bonner, R. M. J. Am. Chem. SOC. 1951, 73,2872. (44) Hutchins, R. 0.; Hoke, D.; Keogh, J.; Koharski, D. Tetrahedron

(45) Bell, H. M.; Vanderslice, C. W.; Spehar, A. J. Org. Chem. 1969,

(46) Gribble, G. W.; Leese, R. M.; Evans, B. E. Synthesis 1977, 172.

Lett. 1969, 3495.

34, 3923.

678 Energy & Fuels, Vol. 4, No. 6, 1990

Scheme 111

Me-/&$;; H -N HN

4f

Me'" . \ L

'H

0 C02Me

NaBHJFA

Smith and Smith

OH

H - - - C M e Me

11 J 10 C02Me C0,Me

Me--&@-Pr Me&-; H2/Pd-C

DDQ - -N HN H -N HN

Me"' . ' ' Me \ \ \ Et

'H

COZMe CO@e 12

[4-n-Pr,5-Et] homologue (condensed to [n-Pr,Et] throughout), we selected the same Bmph-d for conversion into the corresponding porphyrin. Thus, treatment of the [n-Pr,Et] homologue of Bmpd-d 4f with 10 equiv of NaBH, in dry TFA provided varying amounts of 9- deoxo-2-( 1-hydroxyethy1)-Bmph-d (10) and 9-deoxo-2- vinyl-Bmph-d (11) (Scheme 111). No material was ob- tained that had not been completely reduced to methylene at the 9-position. Gribble found that this method was limited to compounds that were capable of forming rela- tively stable carbocations in acidic media, since benzyl alcohol and a series of aliphatic alcohols afforded little or no reduction product. The 9,lO-dehydro product is probably not formed in major amounts because of its in- stability; quenching of the carbocation with hydride to give the desired compound must be a more favored process than forming the strained exocyclic alkeno ring. In later experiments it was determined that use of a larger excess of NaBH, (in the form of pellets to allow for slower dis- solution in TFA), and extension of the reaction time, gave the 9-deoxo-2-ethyl compound 12 directly. Catalytic hy- drogenation of the vinyl group in 11 proceeded smoothly to give the ethyl compound 12 in quantitative yield. Treatment of 12 with DDQ gave the corresponding por- phyrin 13 in good yield. Complexation with nickel was accomplished by dissolving in chloroform and treating with excess saturated nickel(I1) acetate in methanol47 providing 3c in quantitative yield (Scheme IV).

A by-product in the above DDQ reaction that was ob- served when the material was purified on silica gel was

(47) Fuhrhop, J.-H.; Smith, K. M. In Porphyrins and Metallo- porphyrins; Smith, K. M., Ed.; Elsevier: Amsterdam, 1975; p 798.

Me I

1 4 Figure 1. Structure of the by-product 14 from the DDQ oxidation of the corresponding chlorin, 12, and network of NOE connec- tivities.

6O2Me b02Me 13 3c

material (14) which had been oxidized a t the 10-position to give the corresponding hydroxy compound. The hy- droxylation was established to be a t the 10-position by proton NMR NOE difference experiments. Irradiation of the proton geminal to the hydroxyl group gave NOES a t the other ring position (position 9, as expected) and to the 7a-CH2 and 7b-CH2 positions. If the hydroxyl substituent were at position 9, it would have given an NOE to the 5-ethyl group (not observed) and not to the propionate substituent. Substitution a t any position other than on the exocyclic ring was clearly ruled out because all other signals in the NMR spectrum were unchanged. Figure 1 shows the NOE connectivities established by the experi- ments carried out.

Benzylic oxidation involving DDQ has been observed previously. Lee and Harvey48 were able to oxidize the benzylic positions of a variety of polycyclic arylalkanes using DDQ. Further oxidation of the hydroxy to the corresponding aryl ketone was also observed. Apparently DDQ selectively oxidized our product a t the 10-position because that is where the most stable cation would be formed. There are a number of secondary benzylic posi- tions around the macrocycle, but the 10-position is near a meso carbon and therefore is different from the others. Ponomarev and S h ~ l ' g a ~ ~ noticed that the 10-position of a number of cyclopentanoporphyrins was easily oxidized on the surface of silica gel. They obtained hydroxy- porphyrins such as 14 upon drying preparative silica gel plates after development. I t is possible, then, that the formation of hydroxyporphyrins observed in our work is a combination of the two above factors since they both give the same result.

Having established the pathway to bacterio- petroporphyrin, the complete mixture of methyl 5-ethyl- bacteriopheophorbides d (HPLC trace, Figure 2) was

~

(48) Lee, H.; Harvey, R. G. J . Org. Chem. 1983, 48, 749. (49) Ponomarev, G . V.; Shul'ga, A. M. Khim. Geterotsikl. Soedin.

(Eng. Trans[.) 1984, 19, 389.

Preparation of Bacteriopetroporphyrins Energy & Fuels, Vol. 4, No. 6, 1990 679

Table I. Proton NMR Chemical Shifts (a, ppm) and Assignments of the Nickel(I1) Bacteriopetroporphyrins din C6Da IEt.Et1 (3b) In-Pr.Et1 (3c) li-Bu.Et1 I3d) - . ~. . . . _ - . . . - . I

ref 16 this work ref 16 this work ref 16 this work a-meso H p-meso H d-meso H

;:E } 8-Me 2a-CHz

7a-CH2

7-OMe

2b-CH3

7b-CHz

9XHz 10-CHz

4b-CHZlCH3 4c-CHs

5b-CH3

4a-CHz

5a-CH2

9.99 10.03 9.89

3.39-3.40

3.9113.94 1.84 4.18 2.96 3.54 3.65 4.82 3.9113.94 1.84

4.00 1.93

iqj B

3b

3a

10.00 10.06 9.93

3.40-3.41

3.9213.94 1.84 4.24 2.98 3.54 3.69 4.87 3.9213.94 1.84

4.03 1.94

3d

0 10 20 30 40 0 10 20 30

Retention Volume (mL) Figure 2. Reversed-phase HPLC traces, at a flow rate of 1.0 mL/min with a Waters Associates Z Module, a 4-pm C-18 car- tridge, and a variable-wavelength detector set at 405 nm, of (A) natural mixture of methyl 5-ethylbacteriopheophorbides d using 10% H20/90% methanol and (B) synthetic nickel(I1) bacterio- petroporphyrin methyl esters (3a-d) using 45% H20/55% tet- rahydrofuran. Assignments of methyl bacteriopheophorbides d (trace A) are, from left to right, [4-Et,5-Et], [4-n-Pr,5-Et], [4-i- Bu,8Et], and [4-neoPn,5-Et], respectively.

subjected to the same series of transformations. Results and yields were comparable throughout the series except it was shown that treatment of 4e-h with a larger excess of NaBH4 for an extended time gave directly the 2- ethyl-9-deoxopheophorbide series in 63 % yield. After oxidation to porphyrin and chelation with nickel as before, the homologous series of porphyrins was obtained and the components were separated by semipreparative HPLC. Milligram quantities of each of the three homologues were obtained in this way. The proton NMR data for the synthetic materials show very good agreement when com- pared with those obtained for the natural materials ob- tained by Ocampo et a1.16 (see Table I).

Analysis of NMR NOE Spectra. Although Ocampo et al. performed a complete NOE study, we decided that only sufficient NMR work need be completed in order to confirm their assignments. Irradiation of the 10-CH2 multiplet a t 4.79 ppm gave NOES at 2.95 (corresponding

10.02 10.07 9.91 3.40 3.44 3.40 3.93 1.84 4.21 2.97 3.54 3.66 4.84 3.95 2.34 1.31 4.02 1.93

10.01 10.05 9.88 3.40 3.44 3.37 3.92 1.85 4.16 2.95 3.54 3.65 4.79 3.94 2.34 1.32 4.02 1.93

10.03 10.07 9.91 3.40 3.45 3.40 3.94 1.85 4.21 2.97 3.54 3.68 4.85 3.87 2.70 1.35 4.03 1.94

9.99 9.99 9.81 3.38 3.45 3.31 3.94 1.86 4.17 2.92 3.54 3.58 4.68 3.86 2.87 1.36 3.97 1.91

to the 7b-CH2 of the propionate group), 4.16 (corre- sponding to the 7a-CH2 of the propionate group), and 3.65 (corresponding to the 9-CH2 group of the exocyclic ring). Irradiation of the d-meso proton at 9.88 ppm gave NOEs at 3.37 and 3.40 ppm, peaks corresponding to the 1-Me and 8-Me. The methyl group that does not show an NOE is the 3-Me, the chemical shift of which is 3.44 ppm. Dif- ferentiation between the 8-Me and the 1-Me is possible by irradiation of the 7a-CH2 a t 4.16 ppm. This gave rise to an NOE at 3.37 ppm that can only correspond to &Me. By elimination, therefore, the peak at 3.40 belongs to the 1-Me. Also observed were NOEs at 2.95 ppm, corre- sponding to 7b-CH2, and at 4.79 ppm, corresponding to the 10-CH2. Determination of which triplet is assigned to 2b and which to 5b (1.93 and 1.85 ppm) was accomplished by irradiation of the 9-CH2 multiplet at 3.65 ppm. This gave NOEs at 4.79 (corresponding to the 10-CH2) and a t 1.93 ppm corresponding to the 5b-CH3; by elimination, therefore, the peak at 1.85 ppm belongs to the 2b-CH,. The rest of the peaks could then be assigned unequivocally by decoupling except the for the a- and 0-meso peaks at 10.01 and 10.05 ppm. Since there is no methyl group near the 0-meso proton, irradiation of the 3-Me could distin- guish between them; it would show an NOE to the a-meso proton. Irradiation of the 3-Me peak at 3.44 ppm showed an NOE to 10.01 ppm, which could only be the a-meso proton. Therefore the resonance at 10.05 ppm is assigned to the P-meso proton.

The NOE experiments confirmed the chemical shifts of the CY-, 0-, and 6-meso protons, the 1,3,8 ring methyls, the 7-propionate substituent, the 9- and 10-CH2 groups, and the 2b- and 5b-methyls. The 4b-CH2 and the 4c-CH3 can be assigned by inspection. The only remaining resonances that needed to be characterized were the 2a-, 4a-, and 5a-CH2 groups which overlap each other in the region 3.9-4.0 ppm, and these were distinguished by decoupling experiments. The decoupling experiments also confirmed the assignments of Ocampo et al. Decoupling of the 5b- CH, at 1.93 ppm collapsed the quartet at 4.02 ppm (5a- CHJ. Decoupling of the 2b-Me at 1.85 ppm collapsed the quartet (partially obscured by the 4a triplet) at 3.92 ppm (2a-CH2). Decoupling the 4b-CH2 multiplet at 2.34 ppm collapsed the triplet at 1.32 ppm (4c-CH3) and the triplet at 3.94 ppm that corresponds to the 4a-CH2. Decoupling the 4c-CH3 triplet at 1.32 ppm collapsed the multiplet of the 4b-CH2 at 2.34 ppm.

Figure 3 summarizes these NOE connectivities and de- coupling data. The proton NMR spectrum is shown in Figure 4.

680 Energy & Fuels, Vol. 4, No. 6, 1990

A'

Smith and Smith

&O,Me

Figure 3. Proton NMR (300 MHz) NOE and decoupling con- nectivities for nickel(I1) [%n-Pr,5-Et]-bacteriopetroporphyrin d methyl ester (312). Arrows with no asterisk indicate NOE only; arrows with one asterisk indicate decoupling only; arrows with two asterisks indicate NOE and decoupling.

El Me

- I " ' l " ' I "

PPm Figure 4. Proton NMR spectrum (300 MHz in C&) of nickel(I1) [4-n-Pr,5-Et]-bacteriopetroporphyrin d methyl ester (3c).

Preparation of "Bacteriopetroporphyrins c and e *. Having thus further verified the structures of the petro- porphyrins isolated by Ocampo et a1.,16 we decided to convert the bacteriochlorophylls c (15) (Chart 111) and e (17) (Chart IV) into their corresponding nickel(I1) bac- teriopetroporphyrins. Although petroporphyrins with a methyl group a t the 6-meso position have not yet been isolated, there is no reason why they should not be at some point in the future. If and when these compounds are eventually found in petroleum, their recognition will be facilitated by the availability of synthetic samples. These two Chlorobium chlorophyll series were also readily available from existing bacteria cultures maintained in our laboratory, so they presented a convenient starting point for preparation of the target bacterioporphyrins.

Bacteriochlorophyll c (15), the main chlorophyll com- ponent of the green sulfur bacteria Prosthecochloris aes- tuarii, was first reported in 1953 and characterized by H ~ l t ~ ~ in 1961. The &methyl group was identified by extensive synthetic s t ~ d i e s ~ ~ ~ ~ ~ ~ and spectroscopic stud-

10 8 6 4 2

(50) Morley, H. V.; Holt, A. S. Can. J . Chem. 1961, 39, 755.

Chart 111

Me Me@;: 1 'Id"

N \ H -N

Me'" . ' ' 'H

0 R02C

R5 R.'

15 R = Famesyl, M = Mg (Bacteriochlorophylls-c)

16 R = Me, M = 2H (Methyl Bacteriopheophorbides-c: Bmph-c)

Chart IV

(a) R4 = Et

(b) R4 = n-Pr (c ) R4 = i-Bu

17 R = Famesyl, M = Mg (Bacteriochlorophyll\-e)

18 R = Me, M = 2H (Methyl Bactenopheophorbidew Bmph-e)

ies.24p53*" The complete structures were finally unequiv- ocally determined (including stereochemistries at position 2) for these compounds by Smith et al.55 Like the bac- teriochlorophylls d, the bacteriochlorophylls c (15) and consequently the Bmph-c (16) occur as homologous mix- tures of compounds in which the substituents a t position 4 can be ethyl, n-propyl, or isobutyl, and at position 5 can be methyl or ethyl.

Bacterial cultures of P. aestuarii were grown in 20-L batches according to procedures already described in the l i t e r a t ~ r e . ~ ~ Harvesting of the cells was done by a simple organic solvent extraction of the media with acetone f ether. This was more convenient than other methods such as centrifugation or filtration of the bacterial cells on Celite followed by organic solvent extraction of the collected cells. Not only was this method faster, but more of the chloro- phyll was actually extracted rather than left in the su-

(51) Holt, A. S.; Hughes, D. W.; Kende, H. J.; Purdie, J. W. J. Plant

(52) Kenner, G. W.; Rimmer, J.; Smith, K. M.; Unsworth, J. F. Philos.

(53) Holt, A. S.; Purdie, J. W.; Wasley, J. W. F. Can. J . Chem. 1966,

(54) Smith, K. M.; Unsworth, J. F. Tetrahedron 1975, 31, 367. (55) Smith, K. M.; Craig, G. W.; Kehres, L. A.; Pfennig, N. J . Chro-

Cell Physiol. (Tokyo) 1963,41, 49.

Trans. R. SOC. London, B 1976,273, 367.

44, 88.

matogr. 1983,281, 209.

Preparation of Bacteriopetroporphyrins

Scheme V OH

H+Me ';""

Energy & Fuels, Vol. 4, No. 6, 1990 681

Chart V. Bacteriopetroporphyrins c Resulting from Diagenesis of Bacteriochlorophylls c (15) and e (17)

C02CH3 2 2

Meg:: Me H -N - NaBH4 TFA

Me" . ' ' 'H

0 Me0& l 6

Me

20 +

M e m R 4

[ol M e m W Me Me

M e \ \ \ *R5

U

I Me02C 19

pernatant liquid or filtrate. Evaporation of the extract was foliowed by transesterification and demetalation with sulfuric acid/methanol. Removal of the carotenoids and other unwanted materials by column chromatography on alumina gave the Bmph-c.

Since the NaBH,/TFA method for deoxygenation worked so well for the Bmph-d series, it was decided to follow the same strategy for the Bmph-c series. The re- actions were performed on the entire homologous mixture, with the ultimate goal of separating the products by HPLC a t the end of the reaction sequence. Thus, treatment of the homologous mixture of Bmph-c (16) with an excess of NaBH, in TFA provided the 9-deoxo-2-ethyl mixture 19 in good yield (Scheme V). Quite often, the NMR spectra of the product showed small amounts of the 9-deoxo-2- vinyl compound 20 to be present, so the crude material after workup was hydrogenated over 10% palladized charcoal for several hours. Removal of the catalyst by filtration on Celite and purification on an alumina column gave 19 in 73% yield. The next step in the reaction se- quence was oxidation of 19 into the corresponding por- phyrin 21. Whereas in the case of the deoxygenated Bmph-d, the oxidation to porphyrin with DDQ could be done virtually by titration from a buret, in this case it was considerably more difficult. Treatment of 19 with DDQ was initially done exactly the same way as with the de- oxy-Bmph-d compounds. By dissolving the chlorin in CH2C12 and adding a solution of DDQ in benzene dropwise, it was hoped the oxidation should give the desired por- phyrin. Instead, TLC monitoring showed the reaction quickly produced large amounts of chromatographically polar material and there was as much starting chlorin as porphyrin. I t was thought most likely that DDQ was over-oxidizing the chlorin; after production of the por- phyrin, it was in turn oxidized to the corresponding cation radical. Attempts to quench the proposed cation radical with NaBH, were unsuccessful. Using less than 1 equiv of DDQ gave the same results. The reaction products were separated by alumina chromatography. The starting chlorin and the desired porphyrin ran very close together and in many instances they were not completely separated, even through the use of a very long alumina column and eluting with 25% cyclohexane/75% CH2ClP. Use of a silica gel column or preparative silica gel TLC plates was avoided for fear of causing the same benzylic oxidation at position 10 that was previously observed.

Since it appeared that over-oxidation was taking place, it was decided to try a weaker oxidizing agent. Treatment

R' R'

of 19 with 1,Cbenzoquinone under a variety of conditions did not oxidize the chlorin at all and quantitative recovery of starting material was obtained. Intermediate in oxi- dizing strength between DDQ and 1,4-benzoquinone is p-chloranil. This, too, was tried without much success on the free base chlorin; mostly starting material was re- covered even though the reaction mixture was refluxed overnight in CHC13. I t is knownMl5' that the oxidation potential of porphyrins and chlorins depends on the metal chelated within. The presence of zinc(I1) imparts a higher electron density onto the periphery of the macrocycle, and this facilitates oxidation. Therefore, oxidation with p - chloranil was attempted on the zinc(I1) complex of 19. This succeeded but the reaction was stopped before all the starting material was consumed because TLC indicated that a large quantity of chromatographically polar material was being formed. After demetalation of the zinc(I1) complex with TFA, the best yield of the free base por- phyrin among several attempts was 1590, along with 27% of unreacted starting material. This was unfortunately about the same yield as obtained by treating the free base with DDQ, so there was still a disadvantage here in having to insert and then remove the chelated zinc. DDQ oxi- dation of nickel(I1) complexes gave mostly decomposition products.

When 21 (obtained from the DDQ reaction) was itself treated with DDQ, the same polar compounds were ob- tained. I t seemed, therefore, that the oxidation to por- phyrin occurs quickly, but the resulting porphyrin can be oxidized almost as readily as the starting chlorin. The relative amounts of starting material and desired porphyrin were always about the same. Since, on the basis of nu- merous other attempts to control the oxidation, there seemed to be no better alternative to using DDQ on the free base chlorin, further preparations of the porphyrin were carried out in that way.

After sufficient quantity of porphyrin was collected, nickel(I1) chelation was accomplished by refluxing 21 in chloroform containing saturated Ni(OAc)2/methanol to give the homologous mixture 22 (Chart V). The HPLC trace is shown in Figure 5. Separation of the homologues was performed by reversed-phase semipreparative HPLC, which gave baseline separation. Because of the relatively small amount of the [i-Bu,Et] homologue, it was necessary

(56) Fuhrhop, J.-H. J . Am. Chem. SOC. 1973,95, 5140. (57) Fuhrhop, J.-H. In Porphyrins and Metalloporphyrins; Smith, K.

M., Ed.; Elsevier, Amsterdam, 1975; p 629.

682 Energy & Fuels, Vol. 4, No. 6, 1990 Smith and Smith

22b

I 1 I I

0 10 20 30 40

Retention Volume (mL) Figure 5. Reversed-phase HPLC traces, at a flow rate of 1.0 mL/min with a Waters Associates RCM 8 X 10 Module, a 4-pm (2-18 cartridge, and a variable-wavelength detector set at 405 nm, of nickel(I1) bacteriopetroporphyrin c methyl ester homologues (22a-d) using 45% H20/55% tetrahydrofuran.

to do numerous injections in order to obtain a significant quantity of this compound.

Analysis of NMR NOE Spectra. As with the por- phyrins obtained from the bacteriochlorophyll d series, it was necessary to record NOE difference spectra to estab- lish the peak assignments (particularly for the a- and @-meso peaks and the methyl peaks). It is most convenient to begin analysis of the NOE data by examining the data for compounds other than the [Et,Me] homologue 22a; the a- and P-meso protons in the [Et,Me] homologue both have neighboring methyl and ethyl groups (the ethyls being completely indistinguishable since they have the same chemical shift), so the observed NOEs do not give very much information on their own. For that reason some of the signals for these compounds (particularly [Et,Me]) have been assigned by analogy with the rest of the ho- mologues. Thus we decided to begin the analysis with the [i-Bu,Et] homologue 22d and proceed with the other three in order of descending molecular weight. The NMR peak assignments for these compounds are listed in Table 11.

[i-Bu,Et] Homologue (22d). Irradiation of the 4c-CH3 doublet at 1.19 ppm gave an NOE to the 4b-CHz multiplet at 2.56 ppm. The methyl signal at 3.41 ppm gave no NOE anywhere, making its assignment the 7-OMe. Irradiation of the methyl singlet a t 3.52 ppm gave NOEs at both 3.13 and 3.16 ppm. Conversely, independent irradiation of the 3.13 and 3.16 ppm singlets both gave an NOE to the 3.52 ppm singlet. Therefore, the peak at 3.52 ppm is the 6- methyl and those a t 3.13 and 3.16 ppm are the 1- and 3-methyls. Distinguishing between these two methyls, however, had to be accomplished in the next experiment.

Irradiation of the 7a-CH, at 4.12 ppm gave NOEs to the multiplet at 4.74 ppm (10-CH,), the triplet a t 2.83 ppm (7b-CHz), and the methyl singlet at 3.16 ppm. Therefore, the 3.16 ppm resonance is the 8-Me, and by elimination, that a t 3.13 ppm is the 1-Me. Irradiation of the signal at 2.83 ppm (7b-CHz) gave NOEs to 4.12 (7a-CH2) and 4.74

Table 11. Proton NMR Chemical Shifts (6, ppm) and Assignments of the Nickel(I1) Bacterioporphyrins c in

CaDa" - - [Et,Me] [Et,Et] [n-Pr,Et] [i-Bu,Et]

(228) (22b) (22c) (22d) 1-Me 3.12 (s) 3.12 (s) 3.12 (9) 3.13 (9) 2a-CH2 3.72 (4) 3.72 (q) 3.72 (q) 3.73 (4) 2b-CH3 1.66 (t) 1.67 (t) 1.66 (t) 1.66 (t) 3-Me 3.20 (s) 3.19 (9) 3.23 (9) 3.24 (9) 4a-CH2 3.72 (4) 3.72 (4) 3.73 (t) 3.66 (d) 4b-CH2/CH3 1.67 (t) 1.67 (4) 2.17 (m) 2.56 (m) 4c-CH3 1.16 (t) 1.19 (d) 5a-CH2/CH3 3.22 (s) 3.80 (q) 3.81 (4) 3.84 (q) 5b-CH3 1.77 (t) 1.78 (t) 1.79 (t) 7a-CHz 4.09 (t) 4.08 (t) 4.09 (t) 4.12 (t) 7b-CH2 2.81 (t) 2.81 (t) 2.81 (t) 2.83 (t) 7-OMe 3.41 (s) 3.41 (s) 3.41 (s) 3.41 (s) 8-Me 3.15 (9) 3.14 (6) 3.14 (s) 3.16 (9) &Me 3.51 (9) 3.49 (8) 3.50 (9) 3.52 (s) 9-CH2 3.45 (m) 3.53 (m) 3.54 (m) 3.55 (m) 10-CH2 4.71 (m) 4.70 (m) 4.71 (m) 4.74 (m) a-meso 9.57 (9) 9.56 (s) 9.58 (s) 9.60 (s) P-meso 9.61 (s) 9.63 (s) 9.65 (s) 9.66 (s)

"s = singlet; q = quartet; t = triplet; m = multiplet.

ppm (10-CH,). The 10-CH, multiplet a t 4.74 ppm gave NO& to 4.12 (7a-CH2), 2.83 (7b-CHz), and 3.55 ppm. The 3.55 ppm signal is the 9-CHz group; it is partially over- lapped with the b-methyl singlet at 3.52 ppm and so when the 3.52 ppm line (b-methyl) was irradiated that a t 3.55 ppm (9-CH2) was also irradiated (unintentionally) giving an NOE to the 10-CH, group.

When the meso proton signal at 9.60 ppm was irradiated, it gave rise to NOEs a t 3.73 ppm and the methyl group at 3.24 ppm. Conversely, irradiation of the 3.24 ppm peak gave an NOE a t 9.60 ppm. Since the P-meso proton does not have a neighboring methyl group, it cannot give this observed NOE. Therefore the 9.60 ppm line is the a-meso proton, and the 3.24 ppm methyl group has to be the 3-Me. Also, the 2a quartet can be assigned to 3.73 ppm. By elimination, the @-proton is a t 9.66 ppm. Irradiation of the P-meso proton at 9.66 ppm gave NOES at 3.66 and 3.84 ppm (4a- and 5a-CH2s). The position of the 4a-CH, quartet was established by simply decoupling the 4b multiplet a t 2.56 ppm and noticing the collapse of the pattern at 3.66 ppm. Since the 3.66 ppm resonance is the 4a-CH,, that a t 3.84 ppm must be the 5a-CH,.

Irradiation of the triplets at 1.66 and 1.79 ppm gave rise to NOEs a t 3.73 and 3.84 ppm, respectively. Decoupling of the two triplets also caused the collapse of the same signals, and the reverse decoupling experiments were also consistent with the observed NOEs. Therefore, the 1.66 ppm resonance is the 2b-Me and that a t 1.79 ppm is the 5b-Me. Figure 6 shows the NOE and decoupling con- nectivities established by these experiments.

[n-Pr,Et] Homologue (22c). The proton NMR spec- trum of 22c is shown in Figure 7. The only difference between this homologue and 22d is that the substituent at position 4 is n-propyl instead of isobutyl. The NOE experiments were done very similarly to those above. Ir- radiation of the methyl singlet at 3.41 ppm gave no NOE anywhere, indicating it to be the 7-OMe. Irradiation of the meso peaks provided the same information as did the previous homologue. Again, since CY and @ have differing neighboring groups (a has an ethyl and a methyl; /3 has an n-propyl and an ethyl), they are easily distinguishable by NOE difference. Irradiation of the meso proton at 9.58 ppm gave an NOE to the methyl singlet at 3.23 ppm and to the quartet at 3.72 ppm, therefore assigning the line at 9.58 ppm as the a-meso proton, that a t 3.23 ppm as the 3-Me, and the 3.72 ppm resonance as the 2a-CHz. (An

Preparation of Bacteriopetroporphyrins ..

n

Energy & Fuels, Vol. 4 , No. 6, 1990 683

are all completely analogous with the assignments made for the [i-Bu,Et] homologue. No crossing over of peaks was observed and the chemical shifts changed only very slightly when moving from the previous homologue to this one. The rest of the assignments, then, were made by simple decoupling experiments and analogy to the previous homologue.

Decoupling the 4a-CH, (whose position was established above by NOE) collapsed the multiplet at 2.17 ppm. Therefore the 2.17 ppm resonance is the 4b-CH2. De- coupling the upfield triplet at 1.16 ppm collapsed the multiplet at 2.17 ppm to a triplet, thus proving the position of the 4c-CH3. Decoupling the triplet at 1.78 ppm col- lapsed the quartet at 3.81 ppm. Since the peak a t 3.81 ppm was shown (by NOE above) to be the 5a quartet, that at 1.78 ppm must belong to the 5b-Me. The triplet cor- responding to 4a-CH, a t 3.73 ppm is partially obscured under the 7-OMe and &methyl peaks, and it disappears when the multiplet at 2.17 ppm is decoupled.

[Et,Et] Homologue (22b). The only difference here is again at the 4-position. However, this only serves to sim- plify the spectrum. NOE and decoupling experiments were performed exactly as for the previous homologue, and there were no unexpected observations. There is again no crossing over of peaks. Although the chemical shifts change very slightly, the relative positions of the methyl and meso peaks does not.

[ Et,Me] Homologue (22a). Distinguishing between some of the signals is difficult for this homologue, even with the use of NOE difference data. Attempts to dis- tinguish the meso protons, for example, by irradiating them and comparing the NOEs to the neighboring groups is uneffective because they give almost the same NOE difference spectra. Both meso protons neighbor a methyl group and an ethyl group. Since the ethyl signals fall on top of each other, they cannot be used to assign the neighboring meso protons. The NOEs to the methyls are different, but unfortunately without a definite assignment of the 3-Me and/or the &Me, they too, are of little value. The only other way to distinguish these methyl groups would be to establish a connectivity between the 9-CHz group and the 5-Me. Although the methyl peaks are well resolved, thus making the experiment easy to perform, the expected connectivity between the 9-CH2 and the 5-methyl was not observed. There is, however, another way the 5-methyl peak could be tentatively assigned. Due to less than complete separation of the homologues by HPLC there is a little [Et,Et] homologue present as an impurity. This makes the signal corresponding to the 5-Me of the [Et,Me] homologue integrate to less than three protons relative to the other methyl peaks. This smaller peak appears a t 3.22 ppm. Further proof of this tentative as- signment is that this shorter peak at this position relative to the other methyl peaks is not observed for the other homologues which have an ethyl substituent a t position 5 instead of a methyl group. If the 5-Me is a t 3.22 ppm, then the 3-Me is at 3.20 ppm, which agrees very well with the observed chemical shift of the 3-Me in the other ho- mologues.

Since the 3- and 5-methyl groups are now distinguished on the basis of the preceding argument, the CY- and p-meso protons and the methyl groups can be distinguished in exactly the same way as described above for the other homologues. The remaining signals are easily assigned by NOEs, decoupling, and analogy.

Two trends were apparent during this analysis which helped in making the assignments of the peaks in this series of proton NMR spectra. (i) In each of the homo-

C02Me

Figure 6. Proton NMR spectrum (300 MHz) NOE and decou- pling connectivities for nickel(I1) [4-n-Pr,S-Et]-bacterio- petroporphyrin c methyl ester (2212). Arrows with no asterisk indicate NOE only; arrows with one asterisk indicate decoupling only; arrows with two asterisks indicate NOE and decoupling.

I( 10 8 6 4 2

PPm Figure 7. Proton NMFt spectrum (300 MHz in C a s ) of nickel(I1) I. n r m . 3 I I . 1 1 . ri t I /an.\ 1+n-rr,a-ac]-DacLeriopetroporpnyrin c memyi ewer [LAC).

NOE is also observed at 9.58 ppm when the peak a t 3.23 ppm is irradiated.) Irradiation of the @-meso proton at 9.65 ppm gave NOEs to the triplet a t 3.73 ppm (4a-CHJ and to the quartet a t 3.81 ppm (5a-CH2). Irradiation of the most downfield methyl singlet (3.50 ppm) gave NOEs to the 2-methyl peaks at 3.12 and 3.14 ppm. Irradiation of these latter two peaks gave NOEs to the 3.50 ppm singlet. Therefore, the line a t 3.50 ppm is the &methyl and the latter two correspond to the 1- and 8-methyls. A small NOE was observed at 3.72 ppm when the 3.12 ppm methyl group was irradiated, indicating the 3.12 ppm peak to be 1-Me, since 8-Me cannot give an NOE to a CH, group. This is not an unexpected observation, but the enhance- ment may be too small to be significant; one would expect that irradiation of the 1-Me could produce an NOE to the 2a-CH2. Irradiation of the other methyl in question did not show the same small NOE, providing further evidence. Also, the assignment of the 1-Me as the peak a t 3.12 ppm and the 8-Me as that at 3.14 ppm is completely analogous to the assignments for the corresponding methyl groups in the [i-Bu,Et] homologue. In fact, all of the assignments made thus far for this compound are not unexpected; they

684 Energy & Fuels, Vol. 4, No. 6, 1990

Scheme VI

HfMe YHO

M#

Smith and Smith

mum growth of bacteria. The harvesting of the bacterio- chlorophylls e, conversion to the corresponding Bmph-e, and isolation of the homologous mixture of Bmph-e pro- cedures were exactly the same as were done for the Bmph-c. The amount of Bmph-e mixture obtained from a 20-L carboy ranged from 184 to 500 mg (i.e., 9.2-25 mg/L of culture).

Several attempts to treat the Bmph-e (18) with NaBH, in TFA under the same conditions as described earlier gave a minute amount of a compound that coeluted on TLC with an authentic sample of 19, along with a large amount of polar baseline material. Since the only difference be- tween Bmph-c and Bmph-e is the 3-formyl group, it was thought possible that reduction of Bmph-e to the 3- hydroxymethyl compound followed by treatment with NaBH,/TFA might give better results. B r o ~ k m a n n ~ ~ found that selective reduction of the 3-formyl group of Bmph-e was possible using NaBH, in wet THF. Thus, treatment of 18 with NaBH, in 10% H20/90% THF at 0 “C for 15 min gave the 3-hydroxymethyl compound 23 (Scheme VI) in an isolated yield of 57 5%. However, when this dihydroxy compound was treated with NaBH4/TFA, it behaved in the same unsatisfactory way as the 3-formyl compound itself. The failure of this reaction should not be a total surprise, because Gribble et al.& found little or no reduction when benzyl alcohol was submitted to these reaction conditions. Therefore, we investigated other methods.

Reduction of the aldehyde and ketone functions with NaBH, proceeded smoothly to give the Bmph-e triol 24.

Me @ / ’ \ \ Rd

Me / ‘M’” ,‘ \N

H -N

Me”’ ,~ ‘ ,\ Et

OH Me02C

24 M = 2 H

25 M = Zn

Attempts to remove the three benzylic hydroxy groups simultaneously by catalytic hydrogenolysis in THF failed. Catalytic hydrogenolysis in the presence of acetic acid or formic acid32 provided minor amounts of a material that coeluted on TLC with an authentic sample of 19 prepared earlier, but the main result was decomposition to polar material. Isolation of the TLC-mobile material was pos- sible, even though it was in very small amount, and the NMR spectra confirmed the identity as 19. However, due to very low yields, a better method was sought. Recently, Lau et al.62 reported reductive deoxygenations of aryl al- dehydes and ketones and allylic, benzylic and tertiary alcohols using Zn12/NaCNBH3 in 1,2-dichloroethane, In comparison with the NaBH,/TFA method, Lau et a1.62 found benzophenone was reduced to diphenylmethane in 95% yield. This method seemed well suited for our pur- poses since 18 contains aryl aldehyde, aryl ketone, and benzylic alcohol functions. Teatment of 18 under the Lau et a1.62 conditions (1.5 equiv of Zn12, 7.5 equiv of NaCN- BH3, in refluxing 1,2-dichloroethane) provided only a mixture of several minor unidentified compounds and, again, only a small amount of the desired material. It was then thought possible that reduction of both the 3-formyl

(62) Lau, C. K.; Dufresne, C.; Belanger, P. C.; Pietre, S.; Scheigetz, J. J. Org. Chem. 1986, 51, 3038.

Me

Me02C \ NaBH4

P H eft‘ Me0,C I 19

THF $HdTFA

Me Me@

Me’ ’:\ Et

H -N

‘H

Me02C 23

R4

cat H 2 1 9 NaBH4 10 - Me

Me02C’ 24

logues the P-meso proton is downfield relative to the CY-

meso proton. (ii) The relative positions of the methyl peaks (from left to right in the spectra) is 6, 7-OMe, (5) 3, 8, 1.

Preparation of “Bacteriopetroporphyrins e “. The bacteriochlorophyll c (15) and e (17) series have the same carbon skeleton except that bacteriochlorophyll e has no 5-methyl homologues; thus, the petroporphyrins that would be expected to be produced from both under geo- logic conditions should be the same. We therefore un- dertook to prepare the 22 homologous series from bac- teriochlorophyll e. It was thought best to take a synthetic route that would intersect the path taken for the bacter- iochlorophyll c as early as possible, making it unnecessary to carry out steps all the way to the porphyrin. It was therefore hoped that using the NaBH,/TFA methodology developed above would provide the deoxo compounds 19 in one step, and the rest of the procedure would be the same and therefore not necessary to carry out. As will be described, the NaBHJTFA methodology did not work satisfactorily so another route had to be devised.

The bacteriochlorophylls e (17) were initially charac- terized by B r o ~ k m a n n . ~ ~ ’ Simpson and Smith deter- mined the correct stereochemistries of the 2-( l-hydroxy- ethyl) group for the homologues.20 Growth of the bac- teriochlorophyll e producing bacteria (Chlorobium pheo- uibroides) was performed according to the literature pro- cedure.20 About 30 days was typically allowed for maxi-

(58) Brockmann, H.; Gloe, A,; Risch, N.; Trowitzsch, W. Liebigs Ann.

(59) Brockmann, H. Philos. Trans. R. SOC. London, B 1976,273, 277. (60) Risch, N.; Brockmann, H. Liebigs Ann. Chem. 1976, 578. (61) Risch, N.; Kemmer, T.; Brockmann, H. Liebigs Ann. Chem. 1978,

Chem. 1976,566.

585.

Preparation of Bacteriopetroporphyrins Energy & Fuels, Vol. 4, No. 6, 1990 685

ethyl)-Bmph-d (10). Sodium borohydride (202 mg; 5.3 mmol; 10 equiv) was carefully added to TFA (20 mL) under a rapid nitrogen flow at 0 "C. The rate of addition was slow enough to allow evolved Hz to be swept away safely, and the temperature of the reaction mixture did not go above 5 "C. This mixture was stirred briefly at 0 OC, and then Bmph-d (300.8 mg; 0.51 mmol) dissolved in TFA (25 mL) was added via a syringe. The reaction was monitored by periodically withdrawing a drop from the re- action mixture, diluting with dichloromethane, and neutralizing with 2-3 drops of triethylamine. This solution was then examined by spectrophotometry. After 4.5 h spectrophotometry showed no residual starting material, so the reaction mixture was poured into a separatory funnel containing water (200 mL) and extracted with CH2C12 until the aqueous layer was colorless. The combined organic layers were washed carefully with saturated aqueous NaHC03 and then three times more with water. The crude mixture was dried over anhydrous Na2S04 and the solvent was evaporated to dryness. The residue was purified by column chromatography on Alumina (Brockmann Grade 111, elution with CH2C12) and provided 9-deoxo-2-vinyl-Bmph-d (1 1) as the fastest running band and then 9-deoxo-2-(l-hydroxyethyl)-Bmph-d (10) as a slower band. The solvents were removed and the residues were crystallized separately from CH2C12/n-hexane, providing yields of 72% and 11% respectively. The yields varied from one reaction to another.

Band 1. 9-Deoxo-2-vinyl-[4-n -Pr,5-Et]-Bmph-d (1 1): mp 157-159 OC; 'H NMR, ppm, 9.95,9.60,8.95 (each s, 1 H, meso-H), 8.29 (dd, 1 H, 2a-H, = 18, Jci, = 12 Hz), 6.36 (d, 1 H, trans-2b-H, J = 18 Hz), 6.16 (d, 1 H, cis-2b-H, J = 12 Hz), 4.8-5.0 (m, 2 H, 10-CHz), 4.67 (m, 1 H, &H), 4.50 (m, 1 H, 7-H), 4.14 (m, 2 H, 9-CH&, 4.05 (q, 2 H, 5a-CH2, J = 7.5 Hz), 3.84 (t, 2 H, 4a-CH2, J = 7.5 Hz), 3.59 (2 overlapping s, 6 H, ring Me and 7-OMe), 3.44 (8 , 3 H, ring Me), 2.25-2.85 (m, 4 H, 7a-CHz and 7b-CHz), 2.22 (m, 2 H, 4b-CHz), 1.94 (t, 3 H, 5b-CH3, J = 7.5 Hz), 1.85 (d, 2 H, &Me, J = 9 Hz), 1.26 (t, 3 H, 4c-CH3, J = 7.5 Hz), -1.59, -3.30 (each br s, 1 H, NH); UV-vis A, (e) 402 (153 loo), 502 (14660), 594 (4380), 650 (38680); MS (FAB), low resolution m/e (%) 563 (64), 562 (loo), 553 (20); MS (FAB), high resolution calcd for C3BH42N402 562.3308, found 562.3300. Anal. Calcd for C3BH42N402: C, 76.48; H, 7.52; N, 9.96. Found: C, 77.06, H, 7.56; N, 10.04.

Band 2. 9-Deoxo-2-( 1-hydroxyethy1)-[a -Pr,Et]-Bmph-d (10): mp 198-299 "C; 'H NMR, ppm, 10.12,9.61,8.92 (each s, 1 H, meso-H), 6.58 (m, 1 H, 2a-H), 4.83-4.92 (m, 2 H, 10-CH2), 4.67 (m, 1 H, 8-H), 4.49 (m, 7-H), 4.12 (m, 9-CH2), 4.04 (q, 2 H, 5a-CHz, J = 7 Hz), 3.84 (t, 2 H, 4a-CHz, J = 7 Hz), 3.58 (8 , 3 H, 7-OMe), 3.55, 3.44 (each s, 3 H, ring Me), 2.54-2.83 (7a-CH2, 7b-CH2, and 2a-OH); 2.33-2.38 (m, 2 H, 4b-CH2), 2.19 (d, 3 H,

8 Me, J = 6 Hz), 1.26 (t, 3 H, 4c-CH3, J = 7 Hz), -1.72, -3.45 (each br s, 1 H, NH); UV-vis A, (e) 395 (165900), 498 (14610), 586 (4570), 642 (42800); MS (FAB), low resolution m/e (%) 581 (M + 1,17), 580 (M', 3), 565 (M - 15,28), 562 (M - 18, loo), 548 (M - 32,32); MS (EI), high resolution calcd for CSHuN4O3 580.3413, found 580.3402. Anal. Calcd for C3BH,N403.0.5Hz0: C, 73.33; H, 7.69; N, 9.52. Found: C, 73.40; H, 7.53; N, 9.53.

Conversion of (10) into (1 1) by Dehydration of the 2 4 1- Hydroxyethyl) Group. 9-Deoxo-Bmph-d (10) (128.2 mg, 0.221 mmol) was dissolved in o-dichlorobenzene (20 mL) and a few milligrams of p-toluenesulfonic acid was added. The mixture was stirred under nitrogen for 35 min at 100 "C after which time TLC indicated no residual starting material. The reaction mixture was poured into water and extracted with CH2ClZ. The organic layer was washed with water once more and then dried over anhydrous N a 8 0 4 and evaporated to dryness. The residue was purified on a column of alumina (Grade 111, elution with CH2C12). The title compound (115.2 mg, 0.205 mmol, 93%) was obtained and was was identical with 11 obtained above by proton NMR and TLC analysis.

2-Ethyl-9-deoxo-[n -Pr,Et]-Bmph-d (12). 9-Deoxo-2-vinyl- Bmph-d (115.2 mg, 0.205 mmol) was dissolved in tetrahydrofuran (30 mL) and stirred over 10% palladmd charcoal (10.4 mg) under H2 overnight (balloon method). The catalyst was then filtered off on Celite. After evaporation of the filtrate the residue was chromatographed on an alumina column, eluting with CH2Clp The title compound was obtained (117.5 mg, 0.208 mmol, 100%

2b-CH3, J = 6 Hz), 1.93 (t, 3 H, 5b-CH3, J = 7 Hz); 1.84 (d, 3 H,

Scheme VI1

10% HCI M e f i R 4

Me >< - Me

Me' H$=+pEt 'H

'H

19 Me0,C 26 )

Me02C

group and the 9-keto group to the corresponding hydroxy groups would facilitate their removal. Thus, the homol- ogous mixture of Bmph-e was reduced to the trihydroxy compound 24 with NaBH4 in a few minutes at room tem- perature. When this was subjected to treatment with Zn12/NaCNBH3 in 1,2-dichloroethane at room tempera- ture, two main compounds (both deoxygenated) were ob- tained: these were the zinc complex 26 and the free base 19.

Since zinc(I1) was inserting (incompletely) during the reaction, we determined it would be best to chelate with zinc(I1) first and then do the reductive deoxygenation in order to obtain only one product. Alternatively, we could have simply removed the zinc from the product by treatment with dilute acid to recover the free base product. Zinc(I1) is both easily inserted and removed, so this extra step would at worst result in only small losses of material in the overall scheme. Thus, 24 was metalated with zinc(I1) by refluxing in CH2C12 with excess Z ~ ( O A C ) ~ in methan01"~ to give the metal complex 25 in 85% yield. Treatment of the zinc(I1) complex with 1.5 equiv of Zn12 and 7.5 equiv of NaCNBH3 in 1,2-dichloroethane at room temperature for 2 h gave the desired deoxygenated zinc complex 26 in 66% yield. Preinsertion of zinc(I1) gave just one product for the deoxygenation, and it also gave a higher yield. Shaking with 10% aqueous HC1 demetalated the zinc(I1) complex quantitatively to give the free base 19 (Scheme VII).

Proton NMR, UV-visible spectra, and analytical TLC were identical for the deoxygenated Bmph-e and the de- oxygenated Bmph-c prepared earlier. At this point the synthetic route converged with the route taken earlier for the Bmph-c series, so it was therefore not necessary to convert compound 19 prepared according to the latter procedure into the porphyrin.

Experimental Section Melting points were measured on a hot-stage apparatus and

were uncorrected. Silica gel 60 (7G230 mesh, Merck) or neutral alumina (Merck; usually Brockmann Grade 111, i.e., deactivated with 6% water) was used for column chromatography. Preparative thin-layer chromatography was carried out on 20 X 20 cm glass plates coated with Merck G 254 silica gel (1 mm thick). Analytical thin-layer chromatography was performed with Merck 60 F254 silica gel (precoated sheets, 0.2 mm thick). Reactions were monitored by thin-layer chromatography and spectrophotometry and were carried out under nitrogen and in the dark. Proton NMR spectra were obtained in deuterochloroform or CsD6 solution at 300 MHz by use of a General Electric QE300 spectrometer; chemical shifts are expressed in ppm relative to chloroform (7.258 ppm). Elemental analyses were performed at the Microchemical Analysis Laboratory, University of Califomia, Berkeley. Electronic absorption spectra were measured in dichloromethane solution with a Hewlett-Packard 8450A spectrophotometer. Mass spectra were obtained on a VG Analytical ZAB-HS instrument. The bacteriochlorophylls c,& d,% and em were obtained from cultures existing in our laboratory and were transformed into the corre- sponding Bmph as described elsewhere.

Nickel(I1) [4-n -Pr,5Et 1-Bacteriopetroporphyrin d. 9- Deoxo-2-vinyl-Bmph-d (11) and 9-Deoxo-2-( l-hydroxy-

686 Energy & Fuels, Vol. 4, No. 6, 1990

yield): mp 149-151 OC; 'H NMR, ppm, 9.80,9.63, 8.90 (each s, 1 H, meso-H), 4.80-5.00 (m, 2 H, 10-CHz), 4.67 (m, 1 H, &H), 4.50 (m, 1 H, 7-H), 4.15 (m, 2 H, 9-CHz), 4.05 (2 overlapping q, 4 H, 2a-CH2 and 5a-CHz), 3.84 (t, 2 H, 4a-CHz, J = 7.5 Hz), 3.57 (s, 3 H, 7-OMe), 3.46, 3.48 (each s, 3 H, ring Me), 2.25-2.85 (m, 4 H, 7a-CHz and 7b-CHz), 2.27 (m, 2 H, 4b-CHz), 1.94 (t, 3 H, 5b-CH,, J = 7.5 Hz), 1.83 (d, 3 H, %Me, J = 9 Hz), 1.80 (t, 3 H,

(each s, 1 H, NH); UV-vis A, (c) 394 (16020% 498 (12800), 586 (4100), 640 (38000); MS (FAB), low resolution m/e (%) 565 (M + 1, loo), 478 (M - 86, 25.6); MS (EI), high resolution calcd for C36H44N402 564.3464, found 534.3436. Anal. Calcd for CMHaN402: C, 76.56 H, 7.85; N, 9.92. Found: C, 76.70; H, 7.88; N, 9.92.

[4-a -Pr,5-Et]-Bacteriopetroporphyrin d (13). 2-Ethyl-9- deoxo-Bmph-a' (68.9 mg, 0.122 mmol) was dissolved in CHzClz (10 mL) and titrated with a solution of 2,3-dichloro-5,6-di- cyanobenzoquinone (DDQ) in benzene. The reaction was very fast, and as it proceeded the color changed from the green of the starting material to gray-green and finally to the red color of the required product. The reaction mixture was immediately poured onto an alumina column and flushed through with CH2C12. TLC indicated there were still some impurities in the product, so it was rechromatographed on a longer column of alumina (Brock- mann Grade 111, eluting with 25% cyclohexane/CHzClp). This provided 54.5 mg (0.097 mmol, 79% yield) of the title compound: mp 214-215 "C; 'H NMR, ppm, 10.02, 9.99, 9.97 (each s, 1 H, meso-H); 5.36 (m, 2 H, 10-CH2), 4.37 (t, 2 H, 7a-CHz), 3.97-4.18 (m, 6 H, 2a-CHz, 4a-CHz, and 5a-CH2 all overlapped, 3.78 (s, 3 H, 7-OMe), 3.68, 3.66, 3.56 (each s, 3 H, ring Me's), 3.11 (t, 2 H, 7b-CH2), 2.34 (m, 2 H, 4b-CHz), 2.00 (t, 3 H, 5b-CH3, J = 7.5 Hz),

Hz),-2.95,-3.7 (each br s, 1 H, NH); UV-vis A,(€) 400 (2240001, 498 (16370), 534 (4120), 564 (6520), 618 (5970); MS, low resolution m / e (%) 562 (loo), 533 (15); MS, high resolution calcd for c36- H42N40z 562.3308; found 562.3331. Anal. Calcd for C36H42N402: C, 76.84; H, 7.82; N, 9.95. Found: C, 76.77; H, 7.63; N, 10.03.

Nickel(I1) [4-a -Pr,5-Et]-Bacteriopetroporphyrin d (3c). Free base porphyrin 13 (33.79 mg, 0.06 mmol) was dissolved in chloroform (20 mL), and a saturated solution of nickel(I1) acetate in methanol (5 mL) was added. The mixture was stirred under reflux for 20 h, and it was then poured into water and diluted with CH2ClP. The organic layer was washed two more times with water, dried over anhydrous NaZSO4, and evaporated to dryness. The residue was chromatographed on an alumina Grade I11 column, eluting with 25% cyclohexane/CHZClz, to give 37.1 mg (0.06 mmol, 100% yield) of the title compound after evaporation; following crystallization from CH2C12/hexane, 27.0 mg (73% yield) was obtained: mp 221-223 OC; lH NMR, ppm (in CDC13), 9.75, 9.74,9.71 (each s, 3 X 1 H, p-meso-H, a-meso-H, and 8-meso-H), 5.05 (m, 2 H, 10-CHz), 4.11 (t, 2 H, 7a-CHz), 3.86-4.00 (m, 8 H, 2a-CHz,5a-CHz,4a-CHz,and 9-CHz), 3.79 (s,3 H,7-OMe),3.49, 3.46, 3.43 (each s, 3 X 3 H, ring methyls), 2.96 (t, 2 H, 7b-CHz); 2.24 (m, 2 H, 4b-CH,), 1.90 (t, 3 H, 2b-CH,, J = 7.5 Hz), 1.26 (t, 3 H, 4c-CH,, J = 7.5 Hz), (in C6D6) 9.95, 9.91, 9.78 (each s, 3 X 1 H, 0-meso-H, a-meso-H, and 8-meso-H), 4.69 (m, 2 H, 10-CHz); 4.06 (t, 2 H, 7a-CHz), 3.82-3.92 (m, 6 H, 2a-CHz, 4a-CHz, and 5a-CHz), 3.55 (m, 2 H, 9-CHz), 3.44 (s, 3 H, 3-Me), 3.30 (s, 3 H, 1-Me), 3.27 (s, 3 H, %Me), 2.85 (t, 2 H, 7b-CH2), 2.25 (m, 2 H,

J = 7.5 Hz), 1.22 (t, 3 H, 4c-CH,, J = 7.5 Hz); UV-vis A,,, (0 394 (217000), 514 (12600), 552 (24190). MS, low resolution m/e (%) 618 (loo), 603 (39), 589 (68); MS, high resolution calcd for C36H40N4Ni0z 618.2505, found 618.2509. Anal. Calcd for C36H40N,NiOz: C, 69.81; H, 6.51; N, 9.05. Found: C, 70.01; H, 6.55; N, 9.16.

Nickel(I1) [4-Et,S-Et]-Bacteriopetroporphyrin d (3b). This compound was obtained by separation from the complete ho- mologous mixture (see text): mp 203-204 OC; 'H NMR, ppm (CDC13), 9.80,9.79,9.78 (each s, 3 X 1 H, meso-H), 5.20 (m, 2 H, 10-CH2), 4.22 (t, 2 H, 7a-CHz), 3.90-4.10 (m, 4 X 2 H, 2a-CH2, 4a-CHz, 5a-CHz, and 9-CHz all overlapped), 3.79 (9, 3 H, 7-OMe), 3.50 (s, 2 X 3 H, ring Me's), 3.48 (6, 3 H, ring Me), 1.92 (t, 3 H, 5b-CH3, J = 7.5 Hz), 1.78, 1.77 (each t, 2 X 3 H, 2b-CH, and 4b-CH3) (for the NMR spectrum in C6D6 see Table I); UV-vis A, (e) 395 (187000), 514 (11 loo), 552 (20900); MS, low resolution

2b-CH3, J = 7.5 Hz), 1.25 (t, 3 H, 4c-CH3, J = 7.5 Hz), -1.70, -3.50

1.85 (t, 3 H, 2b-CH3, J = 7.5 Hz), 1.28 (t, 3 H, 4c-CH3, J = 7.5

4b-CH2), 1.85 (t, 3 H, 5b-CH3, J = 7.5 Hz), 1.75 (t, 3 H, 2b-CH3,

Smith and Smith

m / e (%) 606 (24) 604 (100); MS, high resolution calcd for C35- H38N4Ni02 604.2348, found 604.2343.

Nickel( 11) [4-i-Bu,5-Et]-Bacteriopetroporphyrin d (3d). This compound was obtained by separation from the complete homologous mixture (see text): mp 207-209 OC; 'H-NMR, ppm (CDCl,), 9.77 (s, 1 H, meso-H), 9.75 (s, 2 X 1 H, meso-H), 5.14 (m, 2 H, 10-CHz), 4.17 (t, 2 H, 7a-CH2), 3.91-4.05 (m, 4 X 2 H, 2a-CH2, 4a-CH2, 5a-CHz, and 9-CHz), 3.79 (s, 3 H, 7-OMe), 3.47-3.49 (3s, 3 H, 3 X ring Me's), 2.99 (t, 2 H, 7b-CHz), 2.60 (m,

(d, 6 H, 2 X 4c-CH3's) (for the NMR spectrum in C6D6 see Table I; UV-vis A,,, ( e ) 395 (181300), 514 (10300), 552 (20200); MS (EI), low resolution m/e (%) 634 (74), 633 (41), 632 (loo), 589 (20); MS (EI), high resolution calcd for C37H42N4Ni02 632.2661, found 632.2661.

Nickel(I1) Bacteriopetroporphyrins c. 2-Ethyl-9-deoxo- Bmph-c (E.g., 12). Sodium borohydride (142 mg) was dissolved in TFA (15 mL) at 0 "C under nitrogen. The mixture of Bmph-c homologues (107 mg) was dissolved in TFA (15 mL) and added via a syringe to the NaBH4/TFA solution. After 26 h, with periodic monitoring by spectrophotometry and TLC, the reaction was complete. The mixture was poured into water and extracted with CHzCl,. The organic layer was washed carefully once with saturated aqueous NaHCO,, washed twice with water, dried over anhydrous Na$04, and evaporated to dryness. Proton NMR and TLC analysis of the crude material showed the presence of a small amount of 2-vinyl compound, so the residue was dissolved in tetrahydrofuran and hydrogenated overnight over 10% palladized charcoal. After removal of the catalyst by filtering through Celite, the compound was purified on alumina (Brockmann Grade 111, eluting with CHZClz). The residue did not crystallize well from hexane or MeOH so after evaporation in a small vial and drying in a vacuum oven; 76.6 mg of material was obtained (73% based on molecular weight of the [Et,Et] homologue): 'H NMR, ppm, 9.82 (s, 1 H, a-meso-H), 9.47, 9.46 (s, 1 H, P-meso-H), 4.89 (m, 2 H, 10-CHz), 4.68 (4, 1 H, 8-H), 4.34 (d, 1 H, 7-H), 4.13 (m, 2 H, 9-CHz), 4.05 (s, 3 H, &Me), 4.12-3.97 (m, 4 H, 2a-CHz and 5a-CHz, overlapped by previous 2 signals), 3.83 (m, 2 H, 4a-CHz), 3.55, 3.54, 3.45 (each s, 3 X 3 H, 1-Me, 3-Me,and 7-OMe), 2.57, 2.21 (each m, 4 H, 7-CHzCHz), 1.92 (t, 3 H, 5b-Me), 1.76 (t, 6 H, 2b-Me and 4b-Me), 1.53 (d, 3 H, 8-Me), -0.52, -3.02 (each br s, 1 H, NH); UV-vis A,, (relative absorbances) 402 (1.00), 504 (0.123), 590 (0.059), 644 (0.237). MS, analyzed as components of the natural mixture:

I H, 4b-CH), 1.91 (t, 3 H, 5b-CH3), 1.78 (t, 3 H, 2b-CHJ1 1.24

sample formula calc mass calc M + 1 found

[Et,Me] C35H42N402 550.3308 551.3387 551.3416 [Et,Et] CMHUN4O2 564.3464 565.3543 565.3578 [n-Pr,Et] C,,HGN4O2 578.3621 579.3700 579.3680

9-Deoxo-2-vinyl-Bmph-c (E.g., 11). This compound was obtained as a side product in the above reaction: 'H NMR, ppm, 9.92 (s, 1 H, a-meso-H), 9.42 (s, 1 H, P-meso-H), 8.15 (dd, 1 H, 2a-H, Jtr,, = 17.7, Jcis = 11.7 Hz), 6.25 (dd, 1 H, cis-2b-H, Jcis = 11.7, J,,, = 1.8 Hz), 6.16 (dd, 1 H, trans-2b-H, J,,, = 17.7, Jgem = 1.8 Hz), 4.88 (m, 2 H, 10-CHz), 4.67 (q, 1 H, 8-H), 4.32 (m, 1 H, 7-H), 4.10 (m, 2 H, 9-CHJ, 4.04 (s, 3 H, &Me), 3.98 (q,2 H, 5a-CHz), 3.81 (m, 2 H, 4a-CH,), 3.60, 3.57, 3.40 (each s, 3 X 3 H, 1-Me, 3-Me, and 7-OMe), 2.60, 2.22 (each m, 4 H, 7-CH,CH&, 1.92 (t, 3 H, 5b-CH,), 1.74 (t, 3 H, 4b-CH3), 1.53 (d, 3 H, &Me), -0.37, -2.76 (each br s, 2 X 1 H, NH); UV-vis A,, (relative absorbances) 408 (1.00), 506 (0.127), 596 (0.056), 650 (0.227). MS analyzed as components of the natural mixture:

[i-Bu,Et] C38H48N402 592.3777 593.3856 593.3883

calc sample formula calc mass M + H found

[Et,Me] C36H,,,N402 548.3151 549.3230 549.3239 [Et,Et] CMH42Nd02 562.3308 (563.3387) 562.3333

(563.3348) [n-Pr,Et] C37H14N102 576.3464 577.3543 577.3548

Bacteriopetroporphyrins c (21) via DDQ Oxidation. 9- Deoxo-2-ethyl-Bmph-c (128.5 mg) was dissolved in dry benzene (10 mL) and stirred under nitrogen. DDQ (48.5 mg, <1 equiv) was dissolved in dry benzene (10 mL) and added dropwise to the

[i-Bu,Et] C38H4BN402 590.3621 591.3700 591.3677

Preparation of Bacteriopetroporphyrins Energy & Fuels, Vol. 4, No. 6, 1990 687

for 15 min, the cold solution was poured into water and extracted with CH2C12. The organic layer was washed twice with water, dried over anhydrous Na2S04, and evaporated to dryness. The residue was chromatographed on Brockmann Grade I11 neutral alumina eluting with 2% MeOH/CH2C12 first and then gradually increasing to 5% MeOH/CH2C12 The main band was collected, the solvent was removed and the product was precipitated from CH2C12 with hexane to give 354.9 mg of a microcrystalline green solid (88% based on the molecular weight of the [Et,Et]homo- logue): 'H NMR, ppm, 10.43 (s, 1 H, a-meso-H), 9.61 (s, 1 H, 8-meso-H), 6.72 6.57 (each m, 2 X 1 H, 2a-H and 9-H), 5.92 (m, 2 H, 3-CH2), 5.36,4.72 (m, 2 H, 10-CH2), 4.68 (m, 1 H, 8-H), 4.31 (m, 1 H, 7-H), 4.10 (4, 2 H, 5a-CH2), 4.01 (s, 3 H, &Me), 3.62 (s, 3 H, 7-0Me), 3.92 (q,2 H, 4a-CH2),3.40 (s,3 H, 1-Me), 2.85, 2.67, 2.32 (br s, 3 X OH), 2.56, 2.25 (m, 4 H, 7-CH2CHz), 2.21 (d, 3 H, 2b-Me), 1.99 (t, 3 H, 5b-Me), 1.80 (t, 3 H, 4b-Me [Et,Et]), 1.51 (d, 3 H, &Me), 1.24 (t, 3 H, IC-Me [n-Pr,Et]), -0.36, -2.91 (each br s, 2 X 1 H, NH) (4b of [n-Pr,Et] is obscured); UV-vis A,, (relative absorbances) 410 (LOO), 510 (0.121), 538 (0.063), 592 (0.069), 648 (0.240). MS analyzed as components of the natural mixture:

sample formula calc mass calc M + 1 found

[n-Pr,Et] C37HUIN406 626.3468 627.3547 627.3577 [i-Bu,Et] CzHQN405 640.3625 641.3704 641.3694

Zinc(I1) Bmph-e-triol (25). Bmph-e-triol24 (612.8 mg) was dissolved in CHzClz (150 mL), and saturated zinc(I1) acetate in methanol (10 mL) was added to it. After stirring at reflux for 30 min spectrophotometry and TLC analysis showed the reaction was complete, so it was poured into water and extracted with CH2C12 It was necessary to add a rew milliliters of tetrahydro- furan to enhance the solubility of the product in the organic layer. The organic layer was dried over anhydrous Na2S04 and evapo- rated to dryness. The residue was chromatographed on a Brockmann Grade I11 neutral alumina column, eluting initially with 3.5% MeOH/CH2C12 and then increasing to 5% MeOH/ CHZCl2. The main band was collected and precipitated from CH2C12 with hexane to give 250.2 mg of a microcrystalline blue powder (85% yield based on the molecular weight of the [Et,Et] homologue): lH NMR, ppm (CDC13 + pyridine-d,), 10.12,9.52 (each s, a-meso-H and 0-meso-H), 6.52,6.41 (each m, 1 H, 2a-H and 9-H), 5.87 (m, 2 H, 3-CH2), 5.16 and 4.54 (m, 2 H, 10-CH2), 4.43 (m, 1 H, 8-H), 4.36 (m, 1 H, 7-H), 4.02,3.93 (m, 4 H, 5a-CH2 and 4a-CH2), 3.85 (s, 3 H, &Me), 3.45 (s, 3 H, 7-OMe), 3.43 (s, 3 H, 1-Me), 2.35,2.19 (m, 4H, 7-CH2CH2), 2.11 (d, 3 H, 2b-Me),

8-Me), 1.18 (t, 3 H, 4c-Me [n-Pr,Et]); UV-vis A, (relative ab- sorbances) 414 (1.00), 514 (0.118), 582 (0.113), 622 (0.240). MS analyzed as components of the natural mixture:

samole formula calc mass calc M + 1 found

[Et,Et] CzHMNd05 612.3312 613.3391 613.3397

1.93 (t, 3 H, 5b-CHJ, 1.75 (t, 3 H, 4b-CH3 [Et,Et]), 1.29 (d, 3 H,

Table 111. Proton NMR Chemical Shifts (a, ppm) and Assignments of the Bacteriopetroporphyrins c in CDCl,

~~

[Et,Me] [Et,Et] [n-Pr,Et] [i-Bu,Et] oroton(s) (21a) (21b) (21d (21d) . . . . . , . I . .

a-meso 9.89 (s) 9.88 (s) 9.88 (s) 9.88 (s) j3-meso 9.70 (s) 9.71 (s) 9.70 (s) 9.69 (s) I-Mea 3-Mea 3.45, 3.50, 3.44, 3.50, 3.45, 3.57, 3.46, 2 X

8-Mea 3.61 3.62 3.61 3.61

2a-CH2 b c d e 2b-CH3 1.77 (t) 1.78 (t) 1.78 (t) 1.77 (t) 4a-CH2 b c d e 4b 1.85 (t) 1.86 (t) 2.31 (t) 2.67 (m) 4c-CH3 1.28 (t) 1.27 (d) 5a-CH2/Me 3.57 ( 8 ) c d e 5b-CH3 1.96 (t) 1.97 (t) 1.97 (t) 7a-CH2 4.34 (m) 4.25 (m) 4.35 (m) 4.42 (m) 7b-CH2 3.00 (m) 2.95 (m) 3.00 (m) 3.03 (m) 7d-OMe 3.82 (s) 3.82 (s) 3.82 (a) 3.82 ( 8 ) 6-Me 4.41 (s) 4.35 (s) 4.40 (s) 4.43 (s) 9-CHz b c d e 10-CH2 5.35 (m) 5.28 (m) 5.36 (m) 5.42 (m) NH -1.84, -3.05 -1.89, -3.10 -1.85, -3.05 -1.83, -3.00

(each br s) (each br s) (each br s) (each br s)

Ring methyl singlets not distinguished from each other. *Complex multiplet resulting from the indicated overlapping sig- nals in region 3.97-4.07 ppm, integrated to 6 H. cMultiplet in re- gion 3.94-4.10 ppm, integrated intensity 8 H. dMultiplet in region 3.97-4.10 ppm, integrated intensity 8 H. eMultiplet in region 3.87-4.10 ppm, integrated intensity 8 H.

chlorin via a syringe. After stirring for 10 min, the material was poured immediately onto a Brockmann Grade I11 neutral alumina column and eluted with CH2C12 A large amount of polar baseline material was observed on the column, and the mobile bands (starting material and product) did not separate from each other. These two bands were therefore rechromatographed twice to provide sufficient purity (on alumina Grade I11 eluting with 25% cyclohexane/CHzCl2). Starting material (31.8 mg, 25%) was recovered along with 17.2 mg (14.6%) of the required product. This homologous mixture was separated by HPLC into its com- ponents. Proton NMR spectra are shown in Table 111. UV-vis (for the homologous mixture 21a-d) A,, (relative absorbances) 406 (LOO), 506 (0.116), 540 (0.064), 574 (0.072), 624 (0.056). The products had the following MS characteristics:

sample formula calc mass calc M + 1 found

[Et,Me] CaHa402 548.3151 549.3230 549.3234

[n-Pr,Etl C37HMN402 576.3464 577.3543 577.3527

Nickel(I1) Bacteriopetroporphyrins c (22). The HPLC- separated free base porphyrins (each was in a small amount) were metaiated with nickel(I1) by dissolving in chloroform and adding excess saturated nickel(I1) acetate in methanol. After stirring under nitrogen at reflux overnight, the mixture was diluted with CH2C12 and washed with water three times. Drying over an- hydrous N a 8 0 4 and purification by chromatography on a short alumina Grade I11 column (elution with CH2C12) provided the desired materials in quantitative yields. Proton NMR spectra are shown in Table 11. UV-vis A,, (relative absorbances) (22a) 404 (l.OO), 526 (O.lOO), 564 (0.095); (22b) 404 (l.OO), 524 (0.107), 564 (0.101); (22c) 404 (LOO), 526 (0.099), 564 (0.093); (22d) 404 (LOO), 526 (0.103), 564 (0.098). MS: samole formula calc mass calc M + 1 found

[Et,EtJ CsH42N402 562.3308 563.3387 563.3403

[i-Bu,Et] CsHUIN402 590.3621 591.3700 591.3704

[Et,Me] C35H38N402Ni 604.2348 605.2427 605.2440 [Et,Et] C,Ha402Ni 618.2505 619.2584 619.2606 [n-Pr,Et] C3,Hl2N4O2Ni 632.2661 633.2740 633.2739 [i-Bu,Et] CssHUN4O2Ni 646.2818 647.2897 647.2896

Bmph-e Triol Mixture (24). The homologous mixture of Bmph-e (401.8 mg) was dissolved in methanol (100 mL) and stirred at 0 OC. Sodium borohydride (250 mg) was dissolved in cold methanol (100 mL) and added to the Bmph. After stirring

~~ ~~

[Et,Et] CssH,,N405Zn 674.2447 675.2526 675.2526 [n-Pr,Et] C3,HllN406Zn 688.2603 689.2682 689.2690 [i-Bu,Et] CsHIN405Zn 702.2760 703.2839 703.2820

Bmph-e-diol (23). Bmph-e homologues (50.4 mg) were dis- solved in 10% H20/tetrahydrofuran (15 mL) and stirred at 0 "C. Sodium borohydride (6.7 mg) was also dissolved in 10% H20/ tetrahydrofuran and added to the Bmph-e solution. After 25 min the reaction was shown to be complete by spectrophotometry and TLC analysis, so it was poured into water and extracted with CH2C12. The organic layer was washed with water twice, dried over anhydrous Na2S04, and evaporated to dryness. Chroma- tography on Brockmann Grade I11 neutral alumina, eluting with 1% MeOH/CH2C1,, allowed recovery of 6.0 mg (12%) of starting material. Changing the elution solvent to 5% MeOH/CH2C12 gave a second band which was crystallized from CH2C12/hexane to gve 28.6 mg of the title compound product (57% based on the mo- lecular weight of the [Et,Et] homologue): 'H NMR, ppm, 10.16, 10.12,lO.ll (s, a-meso-H), 9.55,9.54,9.51 (9, 0-meso-H), 6.50 (m, 1 H, 2a-H), 5.77 (s, 2 H, 3-CH2), 5.21 (s, 2 H, lO-CH,), 4.57 (q, 1 H, 8-H), 4.16 (m, 1 H, 7-H), 4.06 (q, 2 H, 5a-CH2), 3.86 (s, 3 H, &Me), 3.75 (q, 2 H, 4a-CH2), 3.58 (s, 3 H, 7-OMe), 3.48 (9, 3 H, 1-Me), 2.48, 2.15 (m, 4 H, 7-CH2CH2), 2.13 (d, 3 H, 2b-Me), 1.93 (t, 3 H, 5b-Me), 1.73 (t, 3 H, 4b-Me [Et,Et]), 1.48 (d, 3 H, 8-Me1,

688 Energy & Fuels 1990, 4 , 688-694

1.20 (t, 3 H, &-Me [n-Pr,Et]), -1.83, (br s, 2 H, NH); UV-vis A, (relative absorbances) 418 (1.00), 522 (0.0861, 5 $4 (0.1051, 608 (0.063), 666 (0.383). MS analyzed as components of the natural mixture:

samole formula calc mass calc M + 1 found

(Et,Et] C3eH42N405 610.3155 611.3234 611.3230

[i-Bu,Et] CaHgN405 638.3468 639.3547 369.3544 [n-Pr,Et] C3,H,,N405 624.3312 625.3391 625.3376

Zinc(I1) 9-Deoxo-2-ethy1-3-methyl-Bmph-e/~ (26). Zinc(I1) Bniph-e-triol (420.8 mg) was dissolved in 1,2-dichloroethane (70 mL). Zn12 (893.3 mg; 1.5 equiv) and then NaCNBH3 (878.2 mg; 7.5 equiv) were added. The reaction was allowed to proceed for 2 h at room temperature. It was then diluted with CH2C12, washed three times with water, dried over anhydrous Na2S04, and evaporated to dryness. The residue was chromatographed on a Brockmann Grade I11 neutral alumina column eluting with 25% cyclohexane/CHzC12. The main band was collected and evapo- rated to give 231 mg of product (66% yield based on molecular weight of the [Et,Et] homologue): 'H NMR, ppm 9.66,9.53 (each s, 2 X 1 H, a-meso-H and /3-meso-H), 4.70 (m, 2 H, 10-CHz), 4.65 (4, 1 H, 8-H), 4.23 (m, 1 H, 7-H), 3.95 (s, 3 H, &-Me), 4.05-3.84 (m, containing 2a-CH2, 4a-CH2, 5a-CH2 and 9-CH,), 2.52,2.20 (m,

7-CH2CHz), 1.90 (t, 3 H, 5b-Me), 1.76, 1.72 (two overlapping q, 6 H, 2b-Me and 4b-Me [Et,Et]), 1.49 (d, 3 H, %Me), 1.24 (t, 3 H, 4c-Me [n-Pr,Et]); UV-vis A, (relative absorbances) 406 (1.00), 512 (0.063), 578 (0.057), 620 (0.210). MS analyzed as components of the natural mixture:

calc samDle formula calc mass M + 1 found

[Et,Et] C36H42N402Zn 626.2599 627.2678 626.2634

[n-Pr,Et] C3,HUN4OZZn 640.2756 641.2835 641.2855 [i-Bu,Et] C~HMN,OzZn 654.2912 655.2991 655.2987

Free Base 9-Deoxo-Bmph-e (19). The zinc(I1) complex was demetalated by shaking with 10% aqueous HC1 for 5 min. It was then washed with water, NaHC03, and twice more with water, dried over anhydrous Na2S04, and evaporated to dryness. The NMR spectrum, UV-vis spectrum, and TLC of this compound were all identical with those of the compound obtained from the deoxygenation of Bmph-c. See compound 19 above.

Acknowledgment. This research was supported by a grant from the National Science Foundation (CHE-86- 19034).

(627.2730)

Derivative Spectrophotometry of Petroporphyrins

David H. Freeman* and Thomas C. O'Haver Department of Chemistry and Biochemistry, University of Maryland,

College Park , Maryland 20742

Received June 11, 1990. Revised Manuscript Received August 20, 1990

Derivative spectroscopy is found to be ideally suited to porphyrin geochemical analysis through numerical differentiation of digitized data provided by diode array spectrophotometry. Choices are made among several derivative and data-averaging algorithms in order to establish proper conformity to porphyrin peak width and to suppress the non-porphyrin background, random noise, and spectral distortion while enhancing the graphic resolution. Illustrative applications of the algorithms are reported. Micropowdered shale (516 pm) was extracted ultrasonically and gave porphyrin assays with *870 relative standard deviation (RSD). Similarly, dilution tests gave concentration ratios with fl70 reproducibility. Derivative extinction coefficients, needed for Beer's law in derivative form, were obtained for Ni2+ and Vrv02+ porphyrin (etio-I) standards in dichloromethane and ethyl acetate with *2% RSD. The resulting gains in analytical precision and speed lead directly toward more reliable study of porphyrin biomarkers.

The petroporphyrins are geological pigments with dis- tinctive rubylike colors. Their analytical determination by spectrophotometry is prone to certain interferences, and its improvement will be considered here. Definitive qualitative analysis for porphyrin pigments is based on X-ray' and NMR2 methods for structure determination. Traces of numerous exocyclic and etioporphyrin-type structures occur in geological extracts as homologous groups3 although an unusual pure metalloporphyrin in crystalline form, a b e l ~ o n i t e , ~ is also known.

(1) Ekstrom, A.; Fookes, C. J. R.; Hambley, T.; Loeh, H. J.; Miller, S.

(2) Sanders, J. K. M.; Waterton, J. C.; Denniss, I. S. J. Chem. SOC.,

(3) Thomas, D. W.; Blumer, M. Ceochim. Cosmochim. Acta 1964,28,

A.; Taylor, J. C. Nature 1983, 306, 173-174.

Perkins Trans. 2 1978, 1150-1157.

1147-1 154.

T h e utility of petroporphyrins for exploring the geo- logical record was linked by Philp to the development of improved analytical technique^.^ Of increasing interest is the finding of distinctive petroporphyrin-precursor re- lationships ascribed to bacterial,6 algal,7-10 and heme"J2

(4) Storm, C.,B.; Krane, J.; Skjetne, T.; Talnaes, N.; Branthaver, J. F.;

(5) Philp, R. P. Mass Spectrosc. Reu. 1985, 4 , 1-54. (6) Ocampo, R.; Callot, H. J.; Albrecht, P. J . Chem. SOC. Chem. Com-

(7) Ocampo, R.; Callot, H. J.; Albrecht, P.; Kintzinger, J. P. Tetra-

( 8 ) Verne-Mismer, J.; Ocampo, R.; Callot, H. J.; Albrecht, P. Tetra-

(9) Verne-Mismer, J.; Ocampo, R.; Callot, H. J.; Albrecht, P. Ibid.

(10) Chicarelli, M. L.; Maxwell, J. R. Ibid. 1984, 25, 4701-4704.

Baker, E. J. Science 1984, 223, 1075-1076.

mun. 1985, 200-201.

hedron Lett . 1984,25, 2589-2592.

hedron Lett . 1988,29, 371-374.

1990, 31, 1751-1754 (Chl b).

0887-0624/90/2504-0688$02.50/0 0 1990 American Chemical Society