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HT115 DE3

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Description

E. coli strain HT115(DE3) has a modified lac promotercontrolling the transcription of T7 RNA polymerase. It is an RNaseIII-deficient E. coli strain with IPTG-inducible T7 polymerase activity

This strain grows on LB or 2xYT plates (and is resistant totetracycline), and competent cells can be made using standard techniques.

Note ontetracycline:

TheTn10 transposon interrupting the rnc14 gene carries a tetracycline resistancegene. Therefore, bacteria should be subjected to tetracycline selection (12.5µg/ml) to maintain the RNase deficiency. However, the transposon is quitestable, as we have not lost it in the absence of selection. Using our protocol(see below and Kamathet al.Genome Biology,2, 1-10) inclusion oftetracycline during feeding significantly decreased the RNAi effect for severalgenes tested, so we recommend that it not be used in culture or in NGM plates duringfeeding using the method below. However, using the method of Timmons,etal.(Gene,263, 103-112), animprovement in feeding results by including tetracycline was reported.

NGMMedia:

Forfeeding plates, use standard NGM agar plus the following ingredients:

Carbenicillinto 25 µg/ml final concentration
IPTG to 1 mM final concentration

Platesare poured fresh 1-3 days before use.

FeedingProtocol(fromKamathet al. (2000) GenomeBiology, 2, 1-10):

1.Pick and grow bacteria 6 hours - overnight (but no longer than 18 hours) in LB+ 50 µg/ml ampicillin, seed onto NGM agar plates including additives (above).(Do not add IPTG or tetracycline to the liquid culture, as this will reduce theRNAi effect.). Bacterial cultures grown shorter times (6 hours) sometimes givebetter results. The lawn quality is improved if the culture is dried quickly byleaving the lids off for about 20 minutes after seeding, but we don't know ifthis affects the RNAi effect. We also have anecdotal evidence that platespoured at least 1 week before use work better than freshly poured plates.


2. Let dry and induce overnight at room temperature.


3. The following day, transfer an L4-stage hermaphrodite onto first plate,minimizing the amount of OP50 bacteria transferred (we usually wash worms in M9buffer and then aliquot them directly onto plates). Leave 72 hours at 15°C (or36-40 hours at 22°C) for RNAi to take effect, then replica plate adult ontoanother plate seeded with the same bacteria. After 24 hours, remove the adultfrom the replica and score the progeny for phenotypes. Alternatively, aliquotembryos or larvae onto the feeding plates and score them later.


4. Note on temperature:
We have observed that some genes give different phenotypes at 15°C vs 22°C;thus, it may be worthwhile to test a given gene using both conditions.

HT115(DE3) genotype
F-, mcrA, mcrB, IN(rrnD-rrnE)1, lambda -, rnc14::Tn10(DE3lysogen: lavUV5 promoter -T7 polymerase) (IPTG-inducible T7 polymerase) (RNaseIII minus).

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pQCXIN,pMSCVpuro,hyg,neo,pBABE-puro,pGH112,pWHM3,pPD49_83,L4440,HT115 DE3,pRevTRE-SV40LargeT,FUW-OSKM,pPYCAGIP,

STOP-eGFP-ROSA26TV

p53-Luc,p27-Luc,pAP1-Luc,pFC-MEKK,pFA2-Elk1,pCDNA5/TO,pBI Tet,pTRE-Tight-Luc,pRevTet-off,on,pGAD424,pGBT9,pACT2 AD,pSos


YCplac22,33,YEplac181,YEplac195,YEplac112,YIplac211,pYRP7,pDR195,pBI101,pCAMBIA1381Z,pCAMBIA1391Z,pSingle-tTS-shRNA,

psiRNAH1-neo,
pSUPER.retro.puro
pSUPER.Retro-GFP/Neo
pAAV-IRES-tdTomato腺相关病毒系统
DB3.1克隆菌株
OmniMAX2 T1 Phage-Resistant Cells克隆菌株
Mach1 T1克隆菌株
XL2-Blue MRF’克隆菌株
XL1-Blue克隆菌株
TOP10克隆菌株
JM110克隆菌株
JM109克隆菌株
pEXP-Lib过表达文库构建载体
pJQ200SK基因置换载体(**型)
pKC1139基因破坏型载体
pOJ260基因破坏型载体
pUG6基因敲除载体
BW25113-aceF-(敲除aceF基因)已敲除基因菌株
BW25113-acnB-(敲除acnB基因)已敲除基因菌株
BW25113-sdhA-(敲除sdhA基因)已敲除基因菌株
BW25113-sucA-(敲除sucA基因)已敲除基因菌株
BW25113-icd-(敲除icd基因)已敲除基因菌株
BW25113-acnA-(敲除acnA基因)已敲除基因菌株
BW25113-fumA-(敲除fumA基因)已敲除基因菌株
BW25113-mdh-(敲除mdh基因)已敲除基因菌株
BW25113-tpiA-(敲除tpiA基因)已敲除基因菌株
BW25113-aceB-(敲除aceB基因)已敲除基因菌株
BW25113-aceA-(敲除aceA基因)已敲除基因菌株
BW25113-aceE-(敲除aceE基因)已敲除基因菌株
BW25113-yjhG-(敲除yjhG基因)已敲除基因菌株
BW25113-xylA-(敲除xylA基因)已敲除基因菌株
BW25113-yjhH-(敲除yjhH基因)已敲除基因菌株
BW25113-yagE-(敲除yagE基因)已敲除基因菌株
BW25113-yagF-(敲除yagF基因)已敲除基因菌株
pCP20基因敲除载体
pKD46基因敲除载体
pKD13基因敲除载体
pKD4基因敲除载体
pKD3基因敲除载体
STOP-eGFP-ROSA26TV基因敲除载体
pPYCAGIP细胞重编程载体
FUW-OSKM细胞重编程载体
pLVX-IRES-ZsGreen1-SV40LargeT细胞永生化载体
pRevTRE-SV40LargeT细胞永生化载体
pPD49_83蠕虫表达载体
pSET152链霉菌整合型载体
pWHM3链霉菌表达载体
pGH112大肠杆菌-链霉菌穿梭载体
pBC-hygro真菌表达载体
pBARGPE1真菌表达载体
pHCMC05大肠杆菌-枯草杆菌穿梭载体
pHCMC02大肠杆菌-枯草杆菌穿梭载体
pHT304大肠杆菌-芽孢杆菌穿梭载体
pGAS-TA-Luc信号通路报告载体
pCRE-Luc信号通路报告载体
pMXs-IRES-GFP逆转录病毒载体
MSCV-IRES-EGFP逆转录病毒载体
pBABE-puro逆转录病毒载体
pRetroX-IRES-ZsGreen1逆转录病毒载体
pRetro-off逆转录病毒载体
pRetro-on逆转录病毒载体
pMSCVpuro逆转录病毒载体
pMSCVhyg逆转录病毒载体
pMSCVneo逆转录病毒载体
pQCXIN逆转录病毒载体
pQCXIH逆转录病毒载体
pLXSN逆转录病毒载体
pLNHX逆转录病毒载体
pLNCX2逆转录病毒载体
pLNCX逆转录病毒载体
pCMV-MCS腺相关病毒系统
pAAV-ZsGreen-shRNA腺相关病毒系统
pAAV-hRK1-IRES-ZsGreen1腺相关病毒系统
pAAV-IRES-ZsGreen1腺相关病毒系统
pAAV-IRES-hrGFP腺相关病毒系统
pAAV-ZsGreen腺相关病毒系统
pAAV-EGFP腺相关病毒系统
pAAV-LacZ腺相关病毒系统
pHelper腺相关病毒系统
pAAV-RC腺相关病毒系统
pAAV-MCS腺相关病毒系统
pcDNA 6.2-GW EmGFP-miRGateway系统
pLenti 6/V5-GW/lacZGateway系统
pLenti 6/TRGateway系统
pcDNA6.2-GWEmGFP-miR negativeGateway系统
pENTR-GusGateway系统
pENTR-GFPGateway系统
pENTR 3CGateway系统
pENTRGateway系统
pYr-adshuttle-6(穿梭载体)(IRES-EGFP结构)腺病毒系统
pYr-adshuttle-4(穿梭载体)(双表达框结构,hEF1αp后已插入EGFP,CMVp后可插入目的基因)腺病毒系统
pYr-adshuttle-3(穿梭载体)(双表达框结构,hEF1αp和CMVp)腺病毒系统
pYr-adshuttle-1(穿梭载体)腺病毒系统
pAd/PL-DEST(骨架载体)腺病毒系统
pDC316-mCMV-tdTomato腺病毒系统
pDC316-mCMV-ZsGreen腺病毒系统
pDC316-mCMV-EGFP腺病毒系统
pDC315腺病毒系统
pAdTrack-TO4腺病毒系统
pAdTrack-CMV腺病毒系统
pAdTrack腺病毒系统
BJ5183(已转化pAdEasy-1载体)配套大肠杆菌
pShuttle腺病毒系统
pBridge酵母三杂交系统
pMyrCytotrap Two-Hybrid System
pSos MAFBCytotrap Two-Hybrid System
pSosCytotrap Two-Hybrid System
AH109配套酿酒酵母
pACT2 AD酵母双杂交系统
pGBT9酵母双杂交系统
pGAD424酵母双杂交系统
EBY100配套酿酒酵母
pRevTet-off四环素调控系统
pRevTet-On四环素调控系统
pRevTRE四环素调控系统
pTK-hyg四环素调控系统
pTRE2 hyg(暂停销售,需验证)四环素调控系统
pTRE2四环素调控系统
pTRE-Tight-Luc四环素调控系统
pTRE-Tight四环素调控系统
pTet-Off四环素调控系统
pTet-on advanced四环素调控系统
pTet-On四环素调控系统
pBI Tet四环素调控系统
pcDNA6/TR四环素调控系统
pCDNA5/TO四环素调控系统
pcDNA4/TO/Myc-His/LacZ四环素调控系统
pcDNA4/TO/Myc-His C四环素调控系统
pcDNA4/TO/Myc-His B四环素调控系统
pcDNA4/TO/Myc-His A四环素调控系统
pFC-MEKK信号通路报告载体
pFA2-Elk1信号通路报告载体
pSRE-Luc信号通路报告载体
pNF-κB-Luc信号通路报告载体
pAP1-Luc信号通路报告载体
p53-Luc信号通路报告载体
pCAT3-Control信号通路报告载体
pGL4.75信号通路报告载体
pGL4.31[luc2P/GAL4UAS/Hygro]信号通路报告载体
pGL4.30[luc2P/NFAT-RE/Hygro]信号通路报告载体
pGL4.29[luc2P/CRE/Hygro

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