2020
DOI: 10.1534/g3.120.401749
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New Strains for Tissue-Specific RNAi Studies in Caenorhabditis elegans

Abstract: RNA interference is a powerful tool for dissecting gene function. In Caenorhabditis elegans, ingestion of double stranded RNA causes strong, systemic knockdown of target genes. Further insight into gene function can be revealed by tissue-specific RNAi techniques. Currently available tissue-specific C. elegans strains rely on rescue of RNAi function in a desired tissue or cell in an otherwise RNAi deficient genetic background. We attempted to assess the contribution of specific tissues to polyunsaturated fatty … Show more

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Cited by 31 publications
(21 citation statements)
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“…pNP165 was obtained by insertion of the dpy-7 promoter, which leads to an epidermal specific expression, in front of VHA-5::GFP into the pNP154 vector. pNP154 was made from a vector containing the SEC cassette for single insertion on Chromosome II at the position of ttTi5605 (pAP087, kindly provided by Ari Pani) (Watts et al, 2020). Constructs were made using Gibson Assembly (NEB Inc., MA) and confirmed by sequencing.…”
Section: Methodsmentioning
confidence: 99%
“…pNP165 was obtained by insertion of the dpy-7 promoter, which leads to an epidermal specific expression, in front of VHA-5::GFP into the pNP154 vector. pNP154 was made from a vector containing the SEC cassette for single insertion on Chromosome II at the position of ttTi5605 (pAP087, kindly provided by Ari Pani) (Watts et al, 2020). Constructs were made using Gibson Assembly (NEB Inc., MA) and confirmed by sequencing.…”
Section: Methodsmentioning
confidence: 99%
“…Because most animals are unaffected, we infer that the rde-1(flexon) allele strongly abrogates rde-1 activity, but the low proportion of escapers suggests that it may not be a true null allele. While there may be some situations in which a low background of residual rde-1 activity may be problematic ( 39 ), we demonstrate below that it is eminently feasible to use rde-1(flexon) for tissue-specific RNAi.…”
Section: Resultsmentioning
confidence: 70%
“…In C. elegans, RNAi is usually performed by feeding worms with bacteria that express double-stranded RNA for a gene of interest ( 37 ). Tissue-specific RNAi has been accomplished by selectively expressing RDE-1/Argonaute in an rde-1 hypomorphic or null mutant background ( 38 , 39 ). As with any other transgenic method, rescue experiments are affected by the strength and specificity of available regulatory regions; for example, our laboratory has had difficulty achieving effective tissue-specific RNAi using ckb-3p or lin-31p to drive RDE-1 expression in an rde-1 null mutant background.…”
Section: Resultsmentioning
confidence: 99%
“…When we knocked down sta-2 expression by RNAi in worms expressing GPA-12*, we observed the expected decrease in the expression of the AMP gene nlp-34 , but a significant increase in the expression of ifas-1 ( Fig 5A ). Similarly, upon infection, knocking down sta-2 specifically in epidermis (in strain IG1502 [ 52 ]) decreased expression of the AMP genes nlp-34 and cnc-2 , but provoked a significant increase in the expression of ifas-1 ( Fig 5B ). In vertebrates, as well as acting as positive regulators of gene expression, STAT proteins can directly repress the accessibility and transcription of specific loci [ 53 ].…”
Section: Resultsmentioning
confidence: 99%