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RiceCAP Virus-Induced Gene Silencing andStable RNAi Workshop
October 31 – November 5, 2005
NOBLETHE SAMUEL ROBERTS
F O U N D A T I O N
The Samuel Roberts Noble Foundation, Inc.Ardmore, Oklahoma
USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Itinerary Location: Samuel Roberts Noble Foundation, Inc.
Ardmore, OK Day 1 (Oct. 30, 2005, afternoon). Arrival, Dinner, Welcome and Opening remarks. Day 2 (Oct. 31, 2005). 1. Lecture: “A Short Review and Considerations When Applying VIGS to Your Research”. (8:15 AM – 9:15 AM, Lablink Conference Room) 2. Linearize and purify plasmids containing Brome mosaic virus (BMV) RNA3 with specific insert sequences provided by participants. 3. Observe VIGS phenotypes in rice plants at 14 days post inoculation with BMV vectors carrying foreign inserts supplied, prior to workshop, by participants. 4. Detect viral RNA in rice leaf tissue infected with BMV vectors using immunocapture RT-PCR. Day 3 (Nov. 1, 2005). 1. Continue immunocapture RT-PCR analysis and evaluate through electrophoresis. 2. In vitro transcription of purified plasmids containing BMV RNA3 with specific insert sequences (plasmid from step 2 on day 2). 3. Lecture on stable RNAi technology, Part I. (1:00 PM – 2:00 PM, Lablink Conference Room) 4. Group picture outside of Kruse Auditorum (2:15 -2:30 PM) 5. Inoculate rice, Nicotiana benthamiana and Chenopodium amaranticolor seedlings with RNA transcripts (from step 2, day 3) and crude extracts prepared from infected N. benthamiana leaves. Day 4 (Nov. 2, 2005) 1. Lecture on stable RNAi technology, Part II. (8:30 AM – 9:30 AM, Lablink Conference Room) 2. Isolate total RNA from leaves of inoculated rice plants at 16 days post inoculation and synthesize cDNA. 3. Prepare for quantitative RT-PCR analysis. Day 5 (Nov. 3, 2005) 1. Analyze gene silencing through semi-quantitative and quantitative RT-PCR. 2. Visualize semi-quantitative RT-PCR results through electrophoresis.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Day 6 (Nov. 4, 2005) 1. Observe VIGS phenotypes in rice plants at 18 days post inoculation with BMV vectors carrying various foreign inserts. 2. Observe local lesions on inoculated C. amaranticolor leaves. 3. Discuss future plans to optimize VIGS technology in monocots using BMV vector. 4. Summary of results from laboratory work. 5. Closing remarks. Day 7 (Nov. 5, 2005) Departure.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Preparation of BMV RNA transcripts for plant inoculation:
1. Mix 43 µl of solution containing 2 µg of template DNA with 5 µl 10x restriction enzyme buffer, 0.5 µl BSA (100 mg/ml, NEB) and 1.5 µl Spe I (p1-11, Buffer 2, NEB) or 1.5 µl PshA I (p2-2, C-BMV RNA3 and C-BMV with insert, Buffer 4, NEB) restriction enzyme. Incubate the tubes at 37 0C for 1.5 h.
2. After incubation, add 50 µl phenol/chloroform/IAA solution to each tube. Vortex
the tubes for 1 min. Spin the tubes at 15000 g for 5 min at RT.
3. Transfer the upper liquid phase into nuclease-free tubes.
4. Add 50 µl chloroform to each tube. Vortex the tubes for 1 min and then spin the tubes at full speed for 5 min.
5. Transfer the upper liquid phase into nuclease-free tubes. Add 5 µl 3 M sodium
acetate, pH 5.2, and 100 µl ice-cold ethanol to each tube. Mix the content and incubate the tubes at –70 0C for 20 min.
6. Centrifuge the tubes at full speed for 15 min and discard the supernatant.
7. Add 0.7 ml ice-cold 70% ethanol to each tube. Flick the tubes several times and
spin them at full speed for 5 min.
8. Discard the supernatant and dry the pellets by spinning the tubes in a SpeedVac for 5 min.
9. Resuspend each pellet in 10 µl nuclease-free H2O. Estimate the concentration of
each linearized plasmid DNA through electrophoresis in a 1% agarose gel.
10. To prepare BMV RNA transcripts from individual linearized plasmid DNA, add 5 µl 2x NTP/CAP solution, 1 µl 10x reaction buffer, 3 µl linearized plasmid DNA (~0.5 µg) and 1 µl T3 enzyme mix into a nuclease-free tube. Mix well.
11. Incubate the tubes at 37 0C for 1.5 h.
12. RNA transcripts obtained can be used immediately to infect plant or store at -70
0C before use.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Immunocapture RT-PCR: Coating tubes with BMV antibody: 1) Dilute BMV antibody in coating buffer (1:5000).
2) Add 30 µl of diluted BMV antibody into a 0.7 ml tube. 3) Incubate the tubes overnight at 4 0C. 4) Wash each tube once with 100 µl of 0.1M phosphate buffer, pH 7.0. 5) Store the tubes at –20 0C before use.
Sample Preparation:
1) Collect tissue from each plant. Grind tissue in 0.1M PB, pH 7.0 (1:10 w/v) in tubes using blue tips attached to a grinder or by hand grinding.
2) Add 30 µl leaf extract to a 0.7 ml tube precoated with BMV antibody. Incubate the
tubes overnight at 4 0C. Reverse Transcription:
1) Wash each tube from overnight incubation with plant extract 3 times with 100 µl of 0.1M PB, pH 7.0.
2) Add 5 µl reverse primer (0.5 µl primer, 25ng/µl, in 4.5 µl H2O) to each tube.
3) Incubate the tubes at 70 0C for 10 min, and then on ice for 2 min. 4) Add 5.0 µl mixed RT reagent to each tube.
1 µl 5 x 1st Strand Buffer 0.5 µl of 0.1 M DTT 0.5 µl of 10 mM dNTP 0.25 µl of RNAsin 0.3 µl Super Script RT 2.25 µl H2O 5.0 µl per tube total
5) Incubate the tubes at 42 0C for 1 hour.
(Page 1, Immunocapture RT-PCR)
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 PCR:
1) Add 19 µl mixed PCR reagent to each new PCR tube.
0.5 µl forward primer 0.5 µl reverse primer 0.4 ul 10 mM dNTP
2.0 µl 10 x PCR buffer 2.0 µl 25 mM MgCl 0.1 µl Taq polymerase 15.0 µl H2O 19.0 µl per tube total
2) Add 2 µl cDNA to each PCR tube and mix. 3) Perform 32 cycles of PCR at 94 0C for 45 sec., 55 0C for 45 sec., 72 0C for 45
sec.
4) Run 1% gel to check the PCR products.
(Page 2, Immunocapture RT-PCR)
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 FES buffer for BMV transcript inoculation (From Scofield et al. (2005) Plant Physiol. 138:2165-2173): 10X GP: 18.77 g glycine (Mallinckrodt) 26.13 g K2HPO4 (Mallinckrodt) (Potassium Phosphate dibasic) Bring volume to 500 ml with ddH20 Autoclave 20 minutes FES 50 ml 10X GP 2.5 g Sodium pyrophosphate (tetrasodium pyrophosphate-Sigma P9146) 2.5 g Bentonite (Fluka 11959) 2.5 g Celite (Fluka 545AW Coarse 22141) Bring volume to 250 ml w/ddH20 (note: bentonite and celite do not dissolve) Shake/vortex prior to adding to transcripts Mix 1 µl RNA1, 1 µl RNA2 and 1 µl RNA3 transcripts with 60 µl FES and inoculate to three rice seedlings. Note: FES was originally from Pogue et al., (1998) Tobamovirus transient expression vector: Tools for plant biology and high-level expression foreign protein in plants. In “Plant Molecular Biology Manual” (S.B. Gelvin and R.A. Schilperoot, Eds.) L4, pp. 1-27. Kluwer Academic Publisgers, Dordrecht, The Netherland.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Plant total RNA extraction:
1) Collect 50 mg leaf tissue from a plant.
2) Grind the tissue in liquid nitrogen and then in 1ml Trizol (GIBCO).
3) Transfer the homogenate into an eppendorf tube and incubate the tube at RT for
5 min.
4) Add 0.2 ml chloroform to each tube and shake sample for 15 sec.
5) Incubate tubes at RT 2 to 3 min.
6) Spin tubes at 12000 g for 15 min at 4 0C.
7) Collect the upper colorless aqueous phase into nuclease-free tubes.
8) Add 350µl Isopropanol to each tube.
9) Incubate the tubes at RT for 10 min and then spin tubes at 12000 g for 10 min at
4 0C.
10) Discard the supernatant and wash the pellets with 75% ethanol (0.7 ml per tube)
11) Spin the tubes at 7500 g for 5 min at 4 0C.
12) Remove supernatant using a pipette, then put tubes on ice with lids open and
allow to air dry for 10 min.
13) Resuspend each pellet in 30 µl nuclease-free H2O.
DNase treatment:
1) Add 1 µl Dnase 1 to 30 µl total RNA.
2) Incubate at 37 C for 15 min.
3) Then incubate at 70 0C for 5 min. Store at -70 0C.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Quantitative PCR (QPCR) analysis for gene expression in rice:
1. Isolate total RNA from leaf tissues of the plants inoculated with buffer only, empty vector and vector with insert, using Trizol reagent (see “Plant total RNA extraction” procedure).
2. Synthesize first strand cDNA from each RNA sample using Oligo dT primer and
Superscript RT as described for semi-quantitative RT-PCR.
3. Design primers for target gene and internal control gene (e.g. Elongation Factor 1α) using Primer Express software (Applied Biosystems). The Tm value of the primers should be 58˚C - 60˚C.
4. For 25 µl QPCR reaction, use 0.5 µl template cDNA, 12.5 µl SYBR Green PCR master
mix (Applied Biosystems) and optimize primer concentrations to give the lowest threshold cycle(CT) and minimum nonspecific amplification by using varying volumes of stock primer (5 µM). Typically, primer volumes should be around 0.5 µl to 1.0 µl.
5. Set up the final QPCR reaction with at least three replicates for each sample. Save the
set up values in the computer and run QPCR reactions using the dissociation protocol. The reactions should also include serial dilutions of cDNA from buffer-inoculated plants for plotting standard curves (e.g.1X, 0.5X, 0.25X, 0.125X and 0.0625X).
6. Analyze QPCR results by standard curve method for relative quantification of gene
expression (see supplementary notes).
Page 1 of QPCR
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Supplementary Notes: Analysis of QPCR results by standard curve method for relative quantification of gene expression Reference: User Bulletin #2- ABI PRISM 7700 Sequence Detection System Constructing a relative standard curve
1. After the QPCR reaction, the results are exported to an Excel spreadsheet by choosing the Export option in the File menu. The exported file contains columns with the sample well number, sample description, standard deviation of the baseline, ∆Rn and CT.
2. Set up three columns in Excel worksheet listing the input amount for the standard curve samples, the log of this input amount, and the CT value.
3. Using the Excel Chart Wizard, draw an XY (scatter) plot on the work sheet with the log input amount as the X values and CT as the Y values. The plotted graph shows the data points in a graphical view.
4. Click one of the data points that appears in graphical view to select it. 5. Open the Insert menu and select Trendline to plot a line through the data point. 6. Go to the Type page and select Linear regression. 7. Go to the Options page and select the boxes for Display Equation on Chart and
display R-squared Value on Chart. 8. Compare your chart with figure1.
y = -2.1404x + 24.35
2 = 0.9875 R
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Figure 1: Standard curve of rice cDNA amplified with actin primers Page 2 of QPCR
19.5 20
20.5 21
21.5 22
22.5 23
CT
0 1 0.5 1.5 2 2.5Log of Quantity
USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Quantification of the input amounts
1. For the line shown in Figure 1, calculate the log input amount by entering the following formula in one cell of the work sheet: = ([cell containing CT value] –b)/m b = y-intercept of standard curve line m = slope of standard curve line Note: In Figure 1, b = 24.35 and m = -2.14 for the equation y = mx + b.
2. Calculate the input amount by entering the following formula in an adjacent cell: = 10^ [cell containing log input amount] Note: The units of the calculated amount are the same as the units used to construct the standard curve.
3. Repeat the steps to construct a standard curve for the endogenous reference (e.g. EF-1α) using the CT values from the results.
4. Because actin and EF-1α are amplified in separate tubes, average the actin and
EF-1α values separately.
5. Divide the amount of actin by the amount of EF-1α to determine the normalized amount of actin.
6. Designate a Calibrator (In our case, the buffer-inoculated plant is the Calibrator),
whose value is approximated as 1.
7. To obtain the results divide the averaged sample value by the averaged calibrator value.
Page 3 of QPCR
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Semi-quantitative RT-PCR: Reverse transcription: Mix 5 µl total RNA (2 µg) 1 µl Oligo dT primer 1 µl 10 mM dNTP 5 µl H2O Incubate the tubes at 70 0C for 5 min. Chill the tubes on ice for 3 min. Add 4 µl 5x 1st strand buffer 2 µl 0.1 M DTT 1 µl RNasin Incubate the tubes at 37 0C for 3 min. Add 1 µl SuperScript RT to each tube. Mix well and incubate the tubes at 37 0C for 1 h followed by 15 min at 70 0C to stop the reaction. PCR: PCR procedure is determined based on the primers and target genes selected by each participant. PCR products are visualized in 1% agarose gel.
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USDA RiceCAP 2005 Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005 Addendum: Isolation of plasmid DNA for in vitro Transcription:
1. Add 1.5 ml cell culture to an eppendorf tube.
2. Centrifuge the tubes at 15000 g for 3 min at RT and pour off the supernatant
while keeping the pellet.
3. Add 0.3 ml Buffer P1 (Qiagen) to each tube, resuspend the pellet and incubate
the tube at RT for 5 min.
4. Add 0.3 ml Buffer P2 (Qiagen) to each tube, mix by inverting the tubes several
times and incubate the tubes on ice for 5 min.
5. Add 0.3 ml 3 M potassium acetate, pH5.5, to each tube, mix by inverting the
tubes several times and incubate the tubes on ice for 15 min.
6. Centrifuge the tubes at 15000 g for 10 min at RT, pour the supernatant into a
clean tube and centrifuge these tubes for 5 min at RT.
7. Pour the supernatant into a clean tube, add 650 µl isopropanol to each tube and
incubate the tubes on ice for 20 min.
8. Centrifuge the tubes at 15000 g for 15 min at RT and pour off the supernatant
while keeping the pellet.
9. Wash the pellet with 0.7 ml 70% ethanol, centrifuge at 15000 g for 5 min at RT.
10. Dry the pellets for 5 min in a SpeedVac.
11. Resuspend each pellet in 20-30 µl TE buffer.
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Sequence or site of interest NucleotideT3 RNA polymerase Promoter sequence 16-32BMV RNA3 32-2152BMV Movement Protein gene 124-1032BMV Coat Protein Gene 1268-1852Hind III restriction site 1953
Note: A portion of the multi-cloning site was deleted (Apa I to EcoRI) was deleted and the ends blunted and ligated, causing the inserted T3 promoter to begin at nucleotide 16 in the vector)
pC-BMV RNA3A/G vector sequence map and reference restriction sites
Virus Induced Gene Silencing and Stable RNAi Workshop
T3 promoter
PshA1
Hind III
Movement Protein Gene
Coat Protein Gene
BMV RNA 3pC-BMV RNA3A/G5112bp
βLa
ctam
ase
pGEM T-EasyBackbone
14
USDA RiceCAP 2005
Virus-Induced Gene Silencing and Stable RNAi Workshop
Samuel Roberts Noble Foundation Ardmore, OK
October 30 – November 5, 2005
A
Primers for Immunocapture RT-PCR: BMV RNA3’ 1490F (forward) 5’-GAATAAGGAGCTTAAGGTCGG-3’ BMV RNA3’ 2119R (Reverse) 5’-CTGGTCTCTTTTAGAGATTTACAGTG-3’
1
A Short Review and Considerations When Applying Virus-Induced Gene Silencing To
Your Research
Richard S. Nelson, Xin Shun Ding, Srinivasa Chaluvadi, Kim Ballard
www.noble.org
Virus-Induced Silencing (VIGS)
Definition: The down-regulation of host gene expression via a virus vector.
- A subcategory of RNA silencing, initiated by virus vectors carrying portions of host genes (Vaistij et al. 2002, Plant Cell, 14:857-867)
- First example: TMV/PDS in N. benthamiana(Kumagi et al. 1995 PNAS 92:1679)
- Host gene can be native or from transgene- Can result in methylation of the host gene leading
to maintenance of silenced state in the absence of the virus initiator, but not always (e.g. Rubisco)
Practical Use: Used for SEQUENCE SPECIFIC and RAPID gene knockout of various host genes (for example; cellulose synthase, Burton et al. 2000 Plant Cell 12:691-705)- Minimum insert size; 23 nt (Thomas et al.,
2001, Plant J. 25; 417), but may depend on virus vector used
- High, but not absolute, sequence specificity for target (generally, about 19 nt stretch with no more than one mismatch within the sequence)
In practice: use more than 100 nts with multiple stretches of 20 nts identity
Virus-Induced Silencing (VIGS) cont.:Virus-Induced Silencing (VIGS) cont.:
VIGS used for both reverse genetic and high throughput forward genetic screens for gene function (reviewed in Burch-Smith et al. 2004 Plant J. 39:734-746)
- forward screens have been facilitated by:
a) expressing the virus vector from a binary vector (35S promoter, ribozyme) through Agrobacterium infiltration
b) “Gatewayize” the virus vector for easy insertion of cDNAs from normalized libraries (can screen thousands of genes in a few months)
Virus Induced Gene SilencingVirus containing host sequence insert Inoculate To Plant:
−Agrobacterium containing virus sequence−Mechanical inoculation of virus
~ 10 days{Symptoms of
virus infection
{{
Virus symptoms
Phenotype after host gene is silenced~ 10 more days
host
Cell
Cell
signal
RNA silencing
DICER (dsRNase)RISC
Modified from Baulcombe, D. (2002) Current Biology 12, R82-84
Viral or Host RDR
Viral or Host RDR
siRNAs
Secondary siRNAs
RDR
RDRRISCDICER
siRNAs
Secondary siRNAs
RDR = RNA dependent RNA polymeraseRISC = RNA-induced silencing complex
2
TRV TRV/actin
DPI: 8 16 24
Actin knockout phenotype on N. benthamiana
Tobacco rattle virus vector courtesy of S. P. Dinesh-Kumar, Yale U.
Comparison of VIGS with other functional genomics approaches:
Method Transformation Gene family analysis Costrequired
VIGS No Yes Low; limited sequencingto ascertain specificity
Chemical No No High; mapping and Mutagenesis sequencing
TILLING No No High; extensive PCRand sequencing
T-DNA insertion Yes No Moderate; sequencingand PCR
Transposon Yes No Moderate; sequencingActivation and PCR
Burch-Smith et al. 2004 Plant J. 39:734
Factors to Consider When Choosing a Virus Vector
Identify a virus that:1) is cloned and available under conditions acceptable to you2) is monopartite, positive sense and forms a rod-shaped virion3) allows inserts of 150 nt or more4) easily infects your favorite host 5) induces mild, systemic symptoms6) enters meristematic tissue (seed transmission may be an
indicator)7) is not vectored by insects, is native to and not considered a
threat to agriculture in the region8) does not encode a strong suppressor of RNA silencing ( see
5 above)
Sampling Of Viruses Reported As Vectors For VIGS In Plants
Virus Genome Host
TRV RNA N. benthamiana, Arabidopsis,
TMV RNA N. benthamiana
PPV RNA N. benthamiana
PVX RNA N. benthamiana
PSbMV RNA P. sativum
TEV RNA N. benthamiana
TYDV DNA P. hybrida
TGMV DNA N. benthamianaTYLCV (DNAβ) DNA L. esculentum, N. tabacum,
L. esculentum
BSMV RNA H. vulgare, T. aestivum
N. glutinosa
PEBV RNA P. sativum
ACMV DNA M. esculenta
CbLCV DNA Arabidopsis
Identification of a VIGS vector for rice
Viruses that naturally infect rice:Virus Composition
Rice black streaked dwarf virus 10 dsRNA segments Rice bunchy stunt virus 12 dsRNA segmentsRice dwarf virus 12 dsRNA segmentsRice gall dwarf virus 12 dsRNA segmentsRice giallume virus 1 ssRNA segmentRice grassy stunt virus 6 ssRNA segmentsRice hoja blanca virus 4 ssRNA segmentsRice necrosis mosaic virus 2 ssRNA segmentsRice ragged stunt virus 10 dsRNA segmentsRice stripe virus 4 ssRNA segmentsRice stripe necrosis virus 4 ssRNA segmentsRice transitory yellowing virus 1 12kb (-) ssRNA segmentRice tungro complex 1 dsDNA/1 ssRNARice yellow mottle virus 1ssRNA segment
Viruses that experimentally infect rice:Foxtail mosaic virus 1 ssRNA segmentSugarcane mosaic virus 1 ssRNA segment
3
Infected Uninfected
Isolation of a virus that infects tall fescue
Xin Shun Ding
John ZwonitzerRouf Mian
Bill Schneider
Electron microscopy shows virus is spherical
Mian et al. (2005) Plant Disease 89:224-227
RNA1 (3.2 kb)m7G
1a (109 kD)
m7G
2a (94 kD)
RNA2 (2.9 kb)
m7G RNA4 (0.9 kb)
CP (20kD)
helmet
pol
m7G
3a (32 kD)
RNA3 (2.1 kb)An
CP
mp
Genome organization of Brome mosaic virus (BMV)
Three genomic RNAs
One subgenomic RNA (RNA 4)
Viruses that naturally infect rice:Virus Composition
Rice black streaked dwarf virus 10 dsRNA segments Rice bunchy stunt virus 12 dsRNA segmentsRice dwarf virus 12 dsRNA segmentsRice gall dwarf virus 12 dsRNA segmentsRice giallume virus 1 ssRNA segmentRice grassy stunt virus 6 ssRNA segmentsRice hoja blanca virus 4 ssRNA segmentsRice necrosis mosaic virus 2 ssRNA segmentsRice ragged stunt virus 10 dsRNA segmentsRice stripe virus 4 ssRNA segmentsRice stripe necrosis virus 4 ssRNA segmentsRice transitory yellowing virus 1 12kb (-) ssRNA segmentRice tungro complex 1 dsDNA/1 ssRNARice yellow mottle virus 1ssRNA segment
Viruses that experimentally infect rice:Foxtail mosaic virus 1 ssRNA segmentSugarcane mosaic virus 1 ssRNA segmentBrome mosaic virus 3 ssRNA segments
Maximizing VIGS Phenotypes
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway CP transgenic plant
RNA1 m7G
m7GRNA2
helmet
pol
F-BMV
F-BMV
m7GSI13’A/G
AnMP
m7GSI13’A/G
An CP
Increasing the length of inducer sequence for VIGS: Trans-complementation in plants using BMV CP or
MP transgenic rice and N. benthamiana
BMV CP and MP transgenic rice plantsare being evaluated
Collaboration with Guo-Liang Wang, Ohio State University
N. benthamiana
RNA3s F-BMV
4
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway
Infected, 200C Infected, 240C Infected, 300C
Mock, 240C
Effect of temperature on PDS Gene Silencing in N. benthamiana Plants
13 dpi
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway
RNA1 m7G
m7GRNA2
helmet
pol
m7GRNA3
Anmp CP
F-BMV
F-BMV
C-BMVAG
….GTATTAATAAUUGAATGTCGAC....
Amino acids different from R-BMV CP sequence
Maximizing Inducer Expression: Genome organization of chimeric BMVAG
Cheng KaoTexas A&M
AAUU modification increases accumulation of RNAs 3 and 4 2.5X
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway
5
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify optimum polarity for insert 4) Identify optimum temperature for phenotype display5) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)6) Minimize virulence of vector7) Identify most responsive target species or cultivar8) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in young plants)9) Modify the host silencing pathway
Modification of BMV vector for Agro-VPI inoculation
pHST40
Dr. Herman B. Scholthof Texas A&M University
RNA1RNA2RNA3
Modification of vascular puncture inoculation (VPI) and Agro-VPI methods for VIGS in rice and other monocots
Rice seed
Rice plant
Now have 30% infection through VPI
To Maximize the VIGS Phenotype:
1) Maximize length of inducer sequence in vector (the more the better rule, e.g. try for >150 bp)
2) Maximize the amount of double-stranded feature in inducer
3) Identify best polarity for insert4) Maximize expression of inducer (e.g. maintenance
of insert in virus genome; accumulation of inducer)5) Minimize virulence of vector6) Identify most responsive target species or cultivar7) Consider tissue specificity of any target sequence
(e.g. can be difficult to obtain VIGS in meristematictissue)
8) Modify the host silencing pathway
Tobacco rattle virus: phytoene desaturase
N. benthamiana has been used extensively as a host for gene knockout analyses through VIGS
0 1.0 2.0 3.0 3.5Nt RDR1
NbRDR1m
NbRdRP1m Contains a 72nt Insert with Tandem In-frame Stop Codons
NtNb
Sequence comparison of cloned NbRDR1m with SA-inducible NtRDR1
NbRdDR1m has 95% identity with NtRDR1
6
Yang et al. PNAS 2004 101:6297-6302
Symptoms on MtRDR1a- expressing and vector control transgenic N. benthamiana plants challenged
with TMV
34 dpi
MtRDR1a-expressor
Vector Control
1-1 1-1 15-1 15-1
23-2 16-223-2 16-2
Lines
Why does VIGS work so well in N. benthamiana?Lu et al., 2003,Methods 30:296a) Greater plasmodesmal exclusion limit (allowing more virus
movement)b) Defective defense components (allowing greater virus
accumulation)
Recent work:In C. elegans, the knockout of RRF-3, encoding an RDR, results
in a mutant that is hypersensitive to RNA silencing due to increased availability of substrate (Simmer et al. 2002 Current Biol. 12:1317-1319).
By analogy, perhaps the knockout of the SA-inducible RdRP from N. benthamiana allows high accumulation of virus RNA which is the indirect substrate for the RDR6 in this plant and subsequent silencing of the target host gene.
Does MtRDR1a expressed in our N. benthamiana plants decrease gene silencing of PDS by competing for substrate going to other NbRDRs ?
PDS silencing phenotype is similar between N. benthamiana expressing or not expressing MtRDR1a
Vector only (-MtRDR1a) +MtRDR1a
TRV-PDS
MtRDR1a does not compete effectively to inhibit gene silencing
Viral RNA accumulation N. benthamiana expressing MtRDR1 after challenge with TMV
Conclusion: MtRDR1a prevents accumulation of virus late in infection, but not early, suggesting that another enzyme in the pathway must be induced to control TMV accumulation
The Cast
Xinshun DingSenior Research
Associate II
Srini ChaluvadiPostdoctoral Associate
Kim BallardResearch Assistant
Support:Samuel Roberts Noble FoundationUSAID/IRRI
1
RNA Interference as a Toolfor Rice Functional Genomics
RiceCAP VIGS and Stable RNAi Workshop
Yinong YangUniversity of Arkansas
• Introduction
• Mechanisms of RNA interference
• Approaches for stable RNAi in plants
• Rice RNAi vectors, protocols and examples
Lecture Outline
I. Introduction
Post-transcriptional gene silencing in plants(Napoli et al. 1990; van der Krol et al. 1990)
Quelling in fungi(Romano and Maciano 1992)
RNA interference in C. elegans(Guo and Kemphues 1995; Fire et al. 1998)
RNA silencing: A brief history
Antiviral mechanism
Cosuppression (post-transcriptional gene silencing)
Discovery of RNAi in Plants
(Baulcombe 2004)(Jorgensen 2003)
Petunia chalcone synthase gene
RNAi: Techniques and Platforms
• Virus delivery (VIGS)• Agroinfection• Biolistic bombardment• Protoplast electroporation
Construct Design Delivery Method
A
B
C
D(Watson et al. 2005)
RNAi: Significance and Application
• Gene silencing at transcriptional (DNA methylationand chromatin modification), post- transcriptional and translational levels
• Regulation of plant growth and development• Regulation of plant response to environmental stimuli
(e.g., antiviral defense and abiotic stress response)
Biological Function:
Powerful Genetic Tool:Gene knockout/knockdown and functional discovery
2
0
3
6
9
CK1
coi1-1coi1-2coi1-3
coi1-4coi1-5coi1-6
coi1-7coi1-8coi1-9coi1-10
coi1-11coi1-12coi1-13coi1-14
coi1-17coi1-18coi1-19
coi1-20coi1-21coi1-22CK2
Suppression of Rice COI1 Expression inTransgenic Lines via RNA Interference
35S Intron NosCOI1COI1
COI1
Rel
ativ
e G
ene
Expr
essi
o n
Insensitivity of Rice coi1 Lines to Jasmonate
0 10 50 100 250 µM MeJA20 20
control coi1-11
* also hypersensitivity to gibberellic acid
Rice coi1 Lines Exhibit a Significant Increaseof Internodal length and Plant Height
CK
coi1-18
coi1-18
coi1-18
CK
CK
Comparison of RNAi with Other Mutagenesis Approaches
• Chemical and radiation mutagenesis• T-DNA insertional mutagenesis and activation tagging• Tos17 retrotransposon mutagenesis• Ac/Ds, Spm transposon mutagenesis
Planned, nonrandom gene silencingSilencing multiple, unrelated genesSilencing redundant genes (multigene family and polyploid)Studying lethal genes via chemical-induced RNAiTissue- and organ-specific gene silencingApplicable for both reverse and forward genetics
Advantages of RNAi in rice functional genomics
II. Mechanisms of RNA Interference
RNAi: A process that converts dsRNA into small RNAsand uses them to direct sequence-specific degradationof cognate single-stranded RNAs.
Silencing trigger: small interfering RNA (siRNA)repeat-associated small interfering RNA (rasiRNA)micro RNA (miRNA)
Silencing target: sequence-specific mRNA cleavagetranslational repressionDNA methylation and transcriptional suppression
RNAi machinery: RNase III endonucleases (Dicer and Drosha)Argonaute (forming RISC or RITS complex)RNA-dependent RNA polymerase (RdRP)
Long dsRNA miRNA precursor
Dicer
siRNA/miRNA duplex (21-27 nt long)
Three RNAi Pathways in Plants
RITSRNA-induced transcriptional silencing complexAt transcriptional level due to DNA methylation
RISC (siRNA-containing)RNA-induced silencing complexAt post-transcriptional level
miRNPmiRNA-containing ribonucleoprotein particleAt translational level
(Meister and Tuschl 2004)
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RNAi machinary
Dicer:long dsRNA-binding and processing
Argonaute:short RNA binding
RNA helicase:RISC assembly
RdRP:RNA amplification, systemic silencing
(Meister and Tuschl 2004)
III. Approaches for Stable RNAi in Plants
1. RNAi Platforms and applications
2. Typical RNAi for silencing a single gene
3. High throughput RNAi (Gateway cloning)
4. High throughput RNAi (SHUTR method)
5. RNAi for multiple, unrelated genes
6. RNAi for redundant genes (multigene family or polyploid)
7. Chemical- or heat-inducible RNAi
8. Tissue- or organ-specific RNAi
Typical RNAi for a Specific Gene
Strong promoter
Gene-specificFragment (>100bp)
Use of intron
(Smith et al. 2000)
High Throughput RNAi (Gateway Cloning)
(Wesley et al. 2001)(Miki and Shimamoto 2004)
PDS: phytoene desaturase gene
High Throughput RNAi (SHUTR Method)
Silencing by heterologous3’ untranslated region
Efficiency: 91%
Effectiveness: 98%
(Brummell et al. 2003)
RNAi for Multiple, Unrelated Genes
(Miki et al. 2005)
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RNAi for Redundant Genes (Multigene Family or Polyploid)
Use of conserved region forsilencing multiple membersof a gene family
(Miki et al. 2005)(Lawrence and Pikaard 2003)
Chemical Inducible RNAi
(Guo et al. 2003)
Heat Inducible RNAi
(Masclaux et al. 2004)
Tissue- or Organ-Specific RNAi
(Byzova et al. 2004)
1st, 2nd whorls 2nd, 3rd whorl
IV. Performing Stable RNAi in Rice
• Rice RNAi vectors: pCambia1300S and pCambia1300RS
• Protocols: construct design and rice transformation
• Examples: verification of gene silencingcharacterization of RNAi transgenic rice
Simple RNAi construct: pCambia 1300S
RNAi Construct Design
High throughput RNAi construct: pCambia 1300RS
2X 35S Int. seq Ter
Antisense Sense
Gene-specific fragmentor conserved region
Typically 200-500 bp(>100 bp)
5
Agrobacterium-Mediated Rice Transformation
C2H4 ETR1, ETR2, ERS1, ERS2
CTR1
EIN3, EIL1, EIL2
EIN2
ERF1
Ethylene responses
Ripening
Senescence
Abscission
Growth inhibition
Hook formation
Wounding responses
Defense responses
Gene activation
Ethylene Signaling Pathway in Arabidopsis
Generation of OsEIN2b Loss of Function Lines
Double-stranded RNA interference
CK-1
CK-2
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 19 20 22 25 29
Suppression of endogenous OsEIN2b
Probed with a sequence region not used for making RNAi construct
CK
Reduced Sensitivity of Rice ein2b Lines to Ethylene
ein2b
0 200 0 200µM ethephon
* No significant difference in ethylene level* Also insensitive to ethylene precursor ACC
EIN2-19CK
EIN2-19
CK
Anthesis time
80
90
100
110
120
130
CK ein2-2 ein2-3 ein2-5 ein2-13 ein2-17 ein2-19 Hyg-
transgenic plants
DA
YS
Late Flowering and Maturation of Rice ein2b Lines
Questions ?
References:
1. Baulcome, D. 2004. RNA silencing in plants. Nature 431: 356-363. 2. Brummell, D., Balint-Kurti, P., Harpster, M.H., Palys, J.M., Oeller, P.W., and Gutterson,
N. 2003. Inverted repeat of a heterologous 3’-untranslated region for high efficiency, high throughput gene silencing. Plant J. 33: 793-800.
3. Byzova, M., Verduyn, C., De Brouwer, D., and De Block, M. 2004. Transforming petals into sepaloid organs in Arabidopsis and oilseed rape: implementation of the hairpin RNA-mediated gene silencing technology in an organ-specific manner, Planta 218: 379–387.
4. Guo, H. S., J. F. Fei, Q. Xie and N. H. Chua, 2003. A chemical-regulated inducible RNAi system in plants, Plant J. 34: 383–392.
5. Jorgensen, R.A. 2003. Sense cosuppression in plants: Past, present, and future. In RNAi: A guide to gene silencing (ed. G.J. Hannon), pp. 5-22. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY.
6. Lawrence and Pikaard. 2003. Transgene-induced RNA interference: a strategy for overcoming gene redundancy in polyploids to generate loss-of-function mutations. Plant journal 36:114-121.
7. Masclaux, F., M. Charpenteau, T. Takahashi, R. Pont-Lezica and J.P. Galaud, 2004. Gene silencing using a heat-inducible RNAi system in Arabidopsis, Biochem. Biophys. Res. Commun. 321: 364–369.
8. Meister, G. and Tuschi, T. 2004. Mechanisms of gene silencing by double-stranded RNA. Nature 431: 343-349.
9. Miki, D. and Shimamoto, K. 2004. Simple RNAi vectors for stable and transient suppression of gene function in rice. Plant Cell Physiol. 45: 490-495.
10. Miki, D., Itoh, R. and Shimamoto, K. 2005. RNA silencing of single and multiple members in a gene family of rice. Plant Physiol. 138: 1903-1913.
11. Napoli, C., Lemieux, C., and Jorgensen, R. 1990. Introduction of chimeric chalcone synthase gene into Petunia results in reversible cosuppression of homologous genes in trans. Plant Cell 2: 279-289.
12. Smith, N. A., Singh, S. P., Wang, M. B., Stoutjesdijk, P. A., Green A.G., and Waterhouse, P.M. 2000. Total silencing by intron-spliced hairpin RNAs. Nature. 407:319–320.
13. Tomari, Y. and Zamore, P.D. (2005) Perspective: machines for RNAi. Genes Dev. 19: 517–529.
14. Watson, J. M., Fusaro, A. F., Wang, M, and Waterhouse, P. M. 2005. RNA silencing platforms in plants. FEBS Letters 579: 5982-5987.
15. Wesley, S.V., Helliwell, C., Smith, N.A., Wang, M-B., Rouse, D., Liu, Q., Gooding, P., Singh, S., Abbott, D., Stoutjesdijk, P. A., Robinson, S. P., Gleave, A. P., Green, A.G. and Waterhouse, P.M. 2001. Constructs for efficient, effective and high throughput gene silencing in plants, Plant J. 27: 581–590.
16. Wielopolska, A., Townley, H., Moore, I., Waterhouse, P. and Helliwell, C. (2005). A high-throughput inducible RNAi vector for plants. Plant Biotech. J. 3: 583-590.
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Mei C., Zhou X., and Y. Yang (in press) Use of RNA interference to dissect defense signaling pathways in rice. In “Plant-Pathogen Interactions: Methods and Protocols” ed. P. Ronald, Humana Press, Inc.
Use of RNA Interference to Dissect Defense Signaling Pathways in Rice Chuansheng Mei, Xiangjun Zhou and Yinong Yang
Summary RNA inference (RNAi) technique is a powerful tool to suppress gene expression
and has been widely used for functional discovery of eukaryotic genes. To dissect defense signal pathways in rice, it is important to generate a series of rice mutant lines deficient in or insensitive to major signal molecules such as jasmonic acid (JA) and ethylene. Here we describe an RNAi protocol for generating and characterizing transgenic gene silencing lines defective in rice JA signaling. The RNAi technique should be useful for effective suppression of host genes encoding signaling components and facilitating the dissection of defense signal pathways in rice.
Key Words
Rice, RNA interference, gene silencing, defense signaling 1. Introduction
RNA interference (RNAi) causes gene-specific silencing based on sequence homology-dependent degradation of cognate mRNA (1, 2). The phenomenon, also known as post-transcriptional gene silencing (PTGS), was first discovered in petunia in which overexpression of the CHS gene encoding a key enzyme (chalcone synthase) in anthocyanin biosynthesis surprisingly resulted in down-regulation of anthocyanin level (3, 4). Recent studies show that RNAi is mediated by short interfering RNAs (siRNAs) or microRNAs (miRNAs), which are resulting from the cleavage of a double-stranded RNA (dsRNA) by an RNase III-related nuclease Dicer (5). RNAi is universally present in plants, animals and fungi, and is now considered as an important mechanism for endogenous gene regulation, development and host defense. Furthermore, the gene silencing method based on RNAi has recently emerged as a powerful tool for functional discovery of eukaryotic genes and genetic engineering of host resistance against viral infection (5,6).
In comparison with T-DNA or transposon insertion, chemical or radiation treatment and other mutagenesis approaches, there are a number of advantages for using RNAi to generate loss-of-function (knockout or knockdown) mutants, especially in a plant species with a large-size genome. First, RNAi allows targeted and effective knockout or
2
knockdown of specific genes at a high frequency without random and laborious screening of loss-of-function mutants from large mutant populations. Second, simultaneous suppression of redundant or homologous genes (e.g., multiple members of a same gene family) can be achieved with RNAi (7). Third, inducible RNAi may provide an effective way for functional analysis of genes whose mutation will lead to embryonic or early developmental lethality (8). Furthermore, a large population of gene silencing lines can be generated through high throughput RNAi (9,10), which will complement other mutagenesis approaches for both forward and reverse genetics-based functional genomic studies.
Stable gene silencing lines can be generated via plant transformation using various RNAi constructs that may include sense, antisense, inverted repeat, or tandem inverted repeat of specific genes. Chuang and Meyerowitz first reported the effective gene silencing in Arabidopsis using an RNAi construct composed of an inverted repeat of the gene of interest (11). Smith et al. proposed to include an intron for more effective gene silencing based on the hypothesis that excision of the intron might improve alignment of the complementary sequences flanking the intron (12). By incorporating a chemical-inducible promoter, Guo et al. constructed an inducible RNAi vector which should be advantageous to the study of lethal genes required for embryo or early development (8). For high efficient, large-scale gene silencing, Wesley et al. developed a high-throughput RNAi vector (pHELLSGATE) by combining with Invitrogen’s Gateway recombination technology (9). With slight modifications, a similar vector (pANDA) was constructed for high-throughput RNAi in rice plants (13). In addition, Brummell et al. developed an innovative method for high-throughput generation of specific RNAi contructs by one-step, simple cloning of any target gene fragment between a 35S promoter and an inverted repeat of a heterologous 3’ untranslated region (10). As a result, a variety of RNAi vectors for different purposes are now available for generating stable gene silencing lines.
During the past decade, significant progress has been made towards the understanding of defense signaling in Arabidopsis, a model dicot. However, little is known about signal transduction and defense pathway interactions leading to host defense response in rice, a model monocot and economically important food crop. Our lab has previously used RNAi to knockout/knockdown rice OsMAPK5 gene encoding a stress-responsive mitogen-activated protein kinase and successfully demonstrated the importance of OsMAPK5 in rice biotic and abiotic signal transduction (14). We have also generated by RNAi a series of transgenic rice lines deficient of or insensitive to major defense signal molecules such as JA and ethylene. These transgenic RNAi lines may serve as powerful genetic tools for epistasis analysis and are important for dissecting defense signal pathways in rice. Here we describe a detailed procedure for generating JA-insensitive transgenic rice lines by RNAi-mediated suppression of a rice orthologue of Arabidopsis COI1 gene (15) that encodes a key component of JA signal transduction.
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2. Materials 2.1. Construction of RNAi Vector
1. Escherichia coli strain DH5α. 2. BamHI, EcoRI, Hind III, KpnI, and SalI restriction enzymes, Taq DNA polymerase
and T4 DNA Ligase. 3. 10 mM dNTPs. 4. 100 bp and 1 kb DNA ladders. 5. pCAMBIA 1300 vector. 6. QIAquick PCR purification kit (Qiagen). 7. QIAprep® Spin miniprep kit (Qiagen). 8. Geneclean III kit (Q-Biogene). 9. Agarose. 10. LB medium (1.0 L): 10 tryptone, 5 g yeast extract, 10 g NaCl, 15 g agar. 11. Ampicillin. 12. Kanamycin.
2.2. Rice Transformation 1. Seeds of rice (Oryza sativa spp. japonica cv. Nipponbare). 2. Agrobacterium tumefaciens strain EHA105 (rifampicin resistant). 3. Bio-Rad MicroPulser Electroporator and cuvette (gap size 2 mm). 4. YEP medium (1.0 L): 10 g Bacto-peptone, 10 g yeast extract, 5 g NaCl, 15 g agar. 5. Chu (N6) basal salt (C1416), MS basal salt (M5524) and MS modified vitamin
powder (M6896) (Sigma). 6. Rifampicin: dissolve in methanol to make 25 mg/mL stock solution and store at -
20°C. 7. Hygromycin B: 50 mg/mL, store at 4°C. 8. Cefotaxime: dissolve in distilled water to make 250 mg/mL stock solution and store
at -20ºC. 9. 1 M acetosyringone stock: dissolve 196.2 mg acetosyringone in 1 mL of DMSO
dimethyl sulfoxide), store at -20ºC. 10. Callus induction medium: 3.98 g Chu (N6) basal salt, 0.1 g MS modified vitamin
powder, 2 mg 2,4-D, 0.5 g casamino acids, 2.5 g proline, 30 g sucrose, and 2 g Gelrite. Adjust pH to 5.7, add water to 1 L, autoclave before use.
11. Suspension medium: 3.98 g Chu (N6) basal salt, 0.1 g MS modified vitamin powder, 0.5 g casamino acids, 30 g sucrose, 10 g glucose, and 100 µM acetosyringone (added after autoclave). Ajust pH to 5.2, add water to 1 L, autoclave before use.
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12. Cocultivation medium: 3.98 g Chu (N6) basal salt, 0.1 g MS modified vitamin powder, 1 g casamino acids, 2 mg 2,4-D, 30 g sucrose, 10 g glucose, 100 µM acetosyringone (added after autoclave), and 2 g Gelrite. Adjust pH to 5.2, add water to 1 L, autoclave before use.
13. Washing medium: 3.98 g Chu (N6) basal salt, 0.1 g MS modified vitamin powder, 30 g sucrose, and 250 mg cefotaxime (added after autoclave). Adjust pH to 5.7, add water to 1 L, autoclave before use.
14. Selection medium: same as the callus induction medium with addition of 250 mg/L cefotaxime and 50 mg/L hygromycin after autoclave.
15. Regeneration medium: 4.31g MS basal salt, 0.1 g MS modified vitamin, 1 g casamino acids, 2 mg kinetin (or 2 mg benzyladenine), 0.1 mg NAA, 30 g sucrose, 30 g sorbitol, 50 mg hygromycin (added after autoclave) and 3 g Gelrite. Adjust pH to 5.7, add water to 1 L, autoclave before use.
16. Rooting medium: 4.31 g MS basal salt, 0.1 g MS modified vitamin, 30 g sucrose, 50 mg hygromycin (added after autoclave), and 2 g Gelrite. Adjust pH to 5.7, add water to 1 L, autoclave before use.
2.3. Analysis of Transgenic Rice Plants
1. TRIzol reagent (Invitrogen). 2. 70% and 100% ethanol. 3. TE buffer: tris-HCl (10 mM), EDTA (1 mM), pH8.0. 4. 3 M sodium acetate, pH 5.2. 5. PerfectHybTM plus hybridization buffer (Sigma). 6. 20X SSC: dissolve 175.3 g of NaCl and 88.2 g of sodium citrate in dH2O, adjust pH
to 7.0 and add water to 1 L. 7. 10% SDS. 8. Nylon membrane. 9. Random primed labeling kit. 10. Formaldehyde. 11. JA. 12. Methyl jasmonate (MeJA).
3. Methods 3.1. Generation of Rice COI1 RNAi Construct
1. Extract genomic DNA from young leaves of rice seedlings using CTAB method as previously described (16).
2. Design two pairs of rice COI1 gene-specific primers containing BamHI/KpnI and BamH/SalI sites, respectively (see Note 1). In order to generate intron-containing hairpin RNA, a 1 kb BamHI/KpnI fragment (A fragement, with a 258 bp COI1 intron)
5
and a 0.7 kb BamH/SalI fragment (B fragment) were amplified from genomic DNA by PCR under the following program: 94°C 2 min; 30 cycles of 94°C 30 sec, 54°C 30 sec, and 72°C 1 min; finally 72°C 10 min (see Note 2).
3. Check the PCR products on 1% agarose gel for specific amplification and verify by restriction enzyme digestion or DNA sequencing as needed.
4. Purify the PCR fragments (A and B) with QIAquick® purification kit. 5. After digested with BamHI and KpnI, the A fragement (~ 1.0 kb, with intron) was
purified with the Geneclean III kit and ligated to the BamHI/KpnI sites of pCAMBIA1300S, which was modified from pCAMBIA1300 and contains a double 35S promoter and a terminator (14).
6. Transform the ligation product into DH5α competent cells by heat shock (42°C, 1 min) treatment. Plate the bacteria on LB medium with kanamycin (50 mg/L) and incubate at 37°C overnight.
7. Pick up 10 bacterial colonies for plasmid DNA extraction using QIAprep® Spin miniprep kit and identify the pCAMBIA1300S recombinant containing the COI1 A fragment by PCR or BamHI/KpnI digestion.
8. Digest the B fragment (~ 0.74 kb) with BamHI and SalI. After purification with the Geneclean III kit, the B fragment was ligated to the BamHI/SalI sites of the above recombinant plasmid. As a result, the final RNAi construct contains two complementary COI1 fragments flanking the COI1 intron, which will allow the formation of inverted repeats or intron-spliced hairpin in rice plants (see Fig. 1A and Note 3).
3.2. Preparation of Agrobacterium Suspension 1. Transform the COI1 RNAi construct into Agrobacterium tumefaciens strain EHA105
using the Bio-Rad MicroPulser electroporator according to the manufacturer’s instruction (see Note 4).
2. Following electroporation, immediately add 1 mL YEP or LB liquid medium to the agrobacterial cells and incubate for 2 hours at 28°C on a shaker.
3. Plate 50-100 µL of agrobacterial suspension onto YEP solid medium containing kanamycin (50 mg/L) and rifampicin (60 mg/L). Incubate the plates at 28°C for two days.
4. Pick up several agrobacterial colonies and identify true transformants carrying the COI1 RNAi construct by PCR and/or restriction digestion. Store the agrobacterial transformant in glycerol stock at -70°C as needed.
5. Streak the agrobacterial transformant on YEP agar medium containing kanamycin (50 mg/L) and rifampicin (60 mg/L) and incubate the plate at 28ºC for 2 days.
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6. Inoculate 1-2 loops of agrobacterial cells into 20 mL YEP liquid medium containing kanamycin (50 mg/L), rifampicin (60 mg/L) and 100 µM of acetosyringone, incubate overnight at 28 ºC on a shaker (150 rpm).
7. Collect overnight agrobacterial cultures (OD600=1-2) in sterile centrifuge tubes by centrifugation (< 3000x g for 10 min).
8. Resuspend agrobacterial cells in 30 ml suspension medium to a density of about OD600=0.05.
3.3. Agrobacterium-Mediated Transformation of RNAi Construct 1. Dehusk 100 immature or mature seeds of rice and surface sterilize with 70% ethanol
for 1 min and then with 50% Clorox (2.6% sodium hypochlorite) for 30 min with gently shaking.
2. Rinse seeds in sterile distilled water three times to remove residual Clorox. 3. Place seeds on the callus induction medium in 10 cm Petri dishes (10 seeds per plate),
seal the plates with parafilm and incubate them under continuous light at 30°C. 4. After two weeks, separate the calli derived from the scutella with scalpel and transfer
them onto fresh callus induction medium and incubate for two more weeks. 5. Select embryogenic calli and soak them in 30 mL agrobacterial suspension
(OD600=0.05) for 30 min with gentle shaking at room temperature. 6. Decant agrobacterial suspension and blot rice calli on sterile filter papers or Kimwipe
tissues to remove excess bacteria. 7. Transfer the inoculated calli onto the cocultivation medium and incubate at 22ºC in
darkness for 2 days. 8. Collect the cocultivated calli in a 50 ml sterile tube; Wash the calli by gentle swirling
for 6 times with sterile 6 x 30 mL dH2O (1-2 min each time), followed by two-time washes (30 min each) with 2 x 30 mL washing medium.
9. Blot the calli on sterile tissue paper to remove excess washing medium. Transfer the calli onto the selection medium and culture under continuous light at 30ºC for three weeks.
10. Transfer hygromycin-resistant calli to the regeneration medium and culture under continuous light at 30ºC.
11. Once shoots are regenerated from calli, transfer them to the rooting medium in test tubes or plastic containers for regeneration of intact rice plantlets.
12. After 2-4 weeks, rice plantlets are ready for transplanting to soil in pots (see Note 5). 3.4. Molecular Characterization of RNAi Transgenic Lines
1. Perform Southern and northern blot analyses to verify the introduction of COI1 RNAi construct into rice transgenic lines and to determine the suppression of endogenous COI1 gene expression, respectively.
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2. Extract genomic DNA from leaves of control and transgenic rice seedlings using the CTAB method (16).
3. Digest 10 µg of genomic DNA with EcoRI in a 30 µL reaction at 37°C overnight. 4. Separate the digested DNA on a 0.8% agarose gel and transfer DNA onto a nylon
membrane according to the standard Southern blot protocol (17). 5. Extract total RNA from leaves of control and transgenic rice seedlings with the
TRIzol reagent by following the manufacturer’s instruction. 6. Separate 15 µg of total RNA on a 1.2% agarose gel containing formaldehyde and
transfer RNA onto a nylon membrane according to the standard northern blot protocol (17).
7. Prepare the B fragment used in the COI1 RNAi construct as a probe for Southern hybridization and the PCR fragment corresponding to 825-1244 nt of rice COI1 gene as a probe for northern hybridization (see Note 6).
8. Radiolabel the above probes with [α-32P] dCTP using the random priming method (17).
9. Hybridize Southern and northern blots in PerfectHybTM plus buffer at 62°C overnight with the radiolabelled probes, respectively.
10. After washing the membranes (2X SSC for 10 min at 62°C twice and then 1X SSC plus 0.5% SDS at 62°C for 20 min twice), the Southern and northern blots are autoradiographed and/or analyzed with a phosphoimager for relative levels of the COI1 gene expression in control plant and RNAi transgenic lines (see Fig. 1B and C).
3.5. Jasmonate Sensitivity Test of COI1 Suppression Lines
1. Collect rice seeds from the control plant and RNAi lines with significant suppression of endogenous COI1 gene.
2. Place surface-sterilized seeds on ½ strength MS medium containing 20 µM MeJA (see Note 7), and incubate at 25°C under the 14-h-light /10- h-dark condition for 9 days.
3. Measure both shoot and root lengths of control and RNAi transgenic seedlings. In comparison with the control, the COI1 suppression lines exhibit less inhibition of shoot growth by MeJA and thus are insensitive to jasmonate (see Note 8).
3.6. Effect of COI1 Suppression on JA-Responsive Gene Expression
1. To determine the role of COI1 in mediating JA signaling, the expression of JA-responsive genes (e.g., OsVSP encoding rice vegetative storage protein, and OsMPK6 encoding a JA-inducible mitogen-activated protein kinase) are examined in response to JA treatment.
2. Spray the leaves of two-week-old control and COI1 RNAi transgenic seedlings with 0.1 mM JA solution.
8
3. Sample water- and JA-treated young leaves at different time points (0, 1, 3, 6, 12, 24 hrs after treatment), freeze them in liquid nitrogen immediately and store at –70°C until use.
4. Extract total RNA from leaf samples and prepare northern blots as described above. 5. Hybridize northern blots with radiolabelled, JA-responsive gene probes (e.g., OsVSP
and OsMPK6). 6. After washing, northern blots are autoradiographed and analyzed with a
phosphoimager for relative expression of JA-responsive genes in control and COI1 suppression lines following JA treatment. Reduced expression of OsVSP and OsMPK6 are observed in the COI1 suppression lines in response to JA treatment, suggesting a positive role of the COI1 in mediating JA-responsive gene expression.
3.7. Disease Resistance Evaluation of RNAi Transgenic Lines
1. Rice RNAi transgenic lines may be evaluated for altered disease resistance and susceptibility using different pathogens such as Magnapothe grisea (rice blast) and Xanthomonas oryzae pv. oryzae (rice bacterial blight), etc.
2. Preliminary tests can be conducted with first generation transgenic lines by spot inoculation of M. grisea on detached leaves (18). Further evaluation of disease resistance should be conducted with heterozygous seeds from the first generation transgenic lines and preferably homozygous seeds identified from the second generation transgenic lines (see Note 9).
3. For the blast infection, two-week-old seedlings are spray-inoculated with M. grisea at a concentration of 250,000 canidial spores/mL. After incubation in a dew chamber (22°C) for 24 hrs, rice plants are moved to a growth chamber and maintained at 28°C with a 14 hr light/10 hr dark cycle.
4. Disease rating as well as measurement of lesion size and number are conducted at six days post-inoculation. The relative growth of M. grisea in control and RNAi transgenic lines can also be determined using a real-time PCR assay or northern blot/phosphoimaging analysis (19).
4. Notes 1. Two pairs of specific primers were designed based on the sequence of rice COI1 gene
(accession number BAB84399). The A fragment, corresponding to 2761-3764 nt (with a 258 bp COI1 intron), was amplified with the first pair of primers (COI1-BamHI-F1, 5’-CCT GGA TCC AGT TAA GTT CCC ACC CAG ATT ATG C; and COI1-KpnI-R, 5’-CCA GGT ACC GGC TAT CCA CAC AGG GTT CTC C). The B fragment, corresponding to 3019-3764 nt, was amplified with the second pair of primers (COI1-BamH I-F2, 5’-CGA GGA TCC GTG AGG AAC GTG ATA GGA
9
GAT AGA GG; and COI1-SalI-R, 5’-CGT GTC GAC GGC TAT CCA CAC AGG GTT CTT CTC C).
2. Gene-specific sequences (e.g., 3’ region) are usually selected for specific gene silencing. The inverted repeat should be at least 100 bp long for effective RNAi. Typically, complementary flanking sequences are 250-500 bp long and separated by a spacer or intron sequence of 200-300 bp. In this case, a 258 bp intron of rice COI1 gene was conveniently included in the RNAi construct since it was reported to improve the effectiveness of RNAi (12).
3. Besides the traditional cloning approach, RNAi construct can be made by high throughput cloning using Gateway recombination technology and inverted repeat of a heterologous 3’-untranslated sequence (9, 10, 13).
4. Alternatively, a freeze-thawed method can be used to introduce the RNAi construct into Agrobacterium cells. Briefly, Agrobacterium competent cells are added with 1 µg plasmid DNA and quickly frozen in liquid nitrogen. The microcentrifuge tubes containing agrobacterial cells were then taken out and immediately put in 37°C water bath for 5 min. After addition of 1 mL YEP liquid medium, incubate the bacterial cells for 2 hours at 28 °C on a shaker before plating.
5. It is important to keep in moisture after transplanting. Transgenic plantlets should be covered with plastic cones or bags for 2-3 days to prevent moisture evaporation and facilitate root growth.
6. In order to detect the endogenous gene expression without the interference of RNAi transgene, the probe used for northern hybridization must be different from the gene sequence region used to make the RNAi construct. If the 3’ region of a gene is used to make RNAi construct, a DNA sequence from the 5’ region should be used as a probe to detect the suppression of endogenous gene expression in northern analysis.
7. MeJA is much less expensive than JA and is adequate for the jasmonate sensitivity test. Although the growth of rice seedlings can be inhibited by MeJA at as low as 1 µM concentration, 20 µM appears to be an appropriate concentration for examining jasmonate insensitivity in rice.
8. Since the seeds from the primary transgenic plants are heterozygous and contain segregants that lose the RNAi transgene, they need to be further analyzed by PCR for the presence or absence of the RNAi transgene after the JA sensitivity test. Based on PCR results, MeJA sensitivity data can be corrected for the genetic segregation. Therefore, it is better to use homozygous seeds from the second generation transgenic plants for JA sensitivity tests.
9. In order to obtain homozygous seeds, rice seeds from the second generation plants should be harvested individually and tested for homozygosity by PCR. In addition, transgene segregation (the presence or absence of RNAi construct) may be detected based on hygromycin sensitivity. Rice seeds and leaf segments can be placed in Petri
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dishes containing 50 mg/L hybromycin solution and tested for inhibition of seed germination or browning of leaf segments, respectively.
References
1. Nishikura, K. (2001) A short primer on RNAi: RNA-directed RNA polymerase acts as a key catalyst. Cell 107, 415-418.
2. Hannon, G. J. (2002) RNA interference. Nature 418, 244-251. 3. Napoli, C., Lemieux, C., and Jorgensen, R. (1990) Introduction of a chimeric
chalcone synthase gene into petunia results in reversible co-suppression of homologous genes in trans. Plant Cell 2, 279-289.
4. van der Krol, A. R., Mur, L. A., Beld, M., Mol, J. N., and Stuitje, A. R. (1990) Flavonoid genes in petunia: addition of a limited number of gene copies may lead to a suppression of gene expression. Plant Cell 2, 291-299.
5. Baulcombe, D. (2004) RNA silencing in plants. Nature 431, 356-363. 6. Fraser, A. G., Kamath, R. S., Zipperlen, P., Martinez-Campos, M., Sohrmann, M.,
and Ahringer, J. (2000) Functional genomic analysis of C. elegans chromosome I by systematic RNA interference. Nature 408, 325-330.
7. Lawrence, R. J. and Pikaard, C. S. (2003) Transgene-induced RNA interference: a strategy for overcoming gene redundancy in polyploids to generate loss-of-function mutations. Plant J. 36, 114-121.
8. Guo, H. S., Fei, J. F., Xie, Q., and Chua, N. H. (2003) A chemical-regulated inducible RNAi system in plants. Plant J. 34, 383-392.
9. Wesley, S. V., Helliwell, C. A., Smith, N. A., Wang, M. B., Rouse, D. T., Liu, Q., Gooding, P. S., Singh, S. P., Abbott, D., Stoutjesdijk, P. A., Robinson, S. P., Gleave, A. P., Green, A. G., and Waterhouse, P. M. (2001) Construct design for efficient, effective and high-throughput gene silencing in plants. Plant J. 27, 581-590.
10. Brummell, D. A., Balint-Kurti, P. J., Harpster, M. H., Palys, J. M., Oeller, P. W., and Gutterson, N. (2003) Inverted repeat of a heterologous 3'-untranslated region for high-efficiency, high-throughput gene silencing. Plant J. 33, 793-800.
11. Chuang, C. F. and Meyerowitz, E. M. (2000) Specific and heritable genetic interference by double-stranded RNA in Arabidopsis thaliana. Proc. Natl. Acad. Sci. USA 97, 4985-4990.
12. Smith, N. A., Singh, S. P., Wang, M. B., Stoutjesdijk, P. A., Green, A. G., and Waterhouse, P. M. (2000) Total silencing by intron-spliced hairpin RNAs. Nature 407, 319-320.
13. Miki, D. and Shimamoto, K. (2004) Simple RNAi vectors for stable and transient suppression of gene function in rice. Plant Cell Physiol. 45, 490-495.
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14. Xiong, L. and Yang, Y. (2003) Disease resistance and abiotic stress tolerance in rice are inversely modulated by an abscisic acid–inducible mitogen-activated protein kinase. Plant Cell 15, 745-759.
15. Xie, D., Feys, B. F., James, S., Nieto-Rostro, M., and Turner, J. G. (1998) COI1: an Arabidopsis gene required for jasmonate-regulated defense and fertility. Science 280, 1091-1094.
16. Chen, D. H. and Ronald, P. C. (1999) A rapid DNA minipreparation method suitable for AFLP and other PCR applications. Plant Mol. Biol. Rep. 17, 53-57.
17. Sambrook, J., Fritsch, E. F., and Maniatis, T. (1998) Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, New York.
18. Jia, Y., Valent, B., and Lee, F. N. (2003) Determination of host responses to Magnaporthe grisea on detached rice leaves using a spot inoculation method. Plant Dis. 87, 129-133.
19. Qi, M. and Yang, Y. (2002) Quantification of Magnaporthe grisea during infection of rice plants using real-time polymerase chain reaction and northern blot/phosphoimaging analyses. Phytopath. 92, 870-876.
Figure legend: Figure 1. Suppression of rice COI1 gene by RNAi. (A) Schematic drawing the COI1 RNAi construct; (B) Southern blot analysis of genomic DNA from the control and COI1 suppression lines after digestion with EcoRI and probed with the B fragment (3019-3764 nt of COI1); (C) Northern blot analysis of total RNAs from the control and COI1 suppression lines. A fragment of 825-1244 nt of COI1 was used as the probe and 25S rRNA was used as the loading control.
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A
B
35S promoter
Kpn I EcoR I
35S polyA
Hind BamH Sal I
Intron 3019-3764nt 3764-3019nt
C
coi1-1coi1-2 coi1-3
COI
rRN
0
20
40
60
80
100C
Kcoi1-17coi1-19coi1-22coi1-4coi1-21coi1-1coi1-11coi1-9coi1-5coi1-18coi1-20coi1-10coi1-3coi1-2coi1-13coi1-14coi1-6coi1-12coi1-7coi1-8
Controloi1-1 coi1-2
Relative ex