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Neither Maternal nor Zygotic med-1/med-2 Genes Play a Major Role in Specifying the Caenorhabditis elegans Endoderm

机译:母本和合子med-1 / med-2基因在确定秀丽隐杆线虫内胚层中均不发挥主要作用

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摘要

The med-1 and med-2 genes encode small, highly similar proteins related to GATA-type transcription factors and have been proposed as necessary for specification of both the mesoderm and the endoderm of Caenorhabditis elegans. However, we have previously presented evidence that neither maternal nor zygotic expression of the med-1/2 genes is necessary to specify the C. elegans endoderm. Contradicting our conclusions, a recent report presented evidence, based on presumed transgene-induced cosuppression, that the med-1/2 genes do indeed show an endoderm-specifying maternal effect. In this article, we reinvestigate med-2(−); med-1(−) embryos using a med-2- specific null allele instead of the chromosomal deficiences used previously and confirm our previous results: the large majority (∼84%) of med-2(−); med-1(−) embryos express gut granules. We also reinvestigate the possibility of a maternal med-1/2 effect by direct injection of med dsRNA into sensitized (med-deficient) hermaphrodites using the standard protocol known to be effective in ablating maternal transcripts, but again find no evidence for any significant maternal med-1/2 effect. We do, however, show that expression of gut granules in med-1/2-deficient embryos is exquisitely sensitive to RNAi against the vacuolar ATPase-encoding unc-32 gene [present on the same multicopy med-1(+)-containing transgenic balancer used in support of the maternal med-1/2 effect]. We thus suggest that the experimental evidence for a maternal med-1/2 effect should be reexamined and may instead reflect cosuppression caused by multiple transgenic unc-32 sequences, not med sequences.
机译:med-1和med-2基因编码与GATA型转录因子相关的小的,高度相似的蛋白质,并已被提议作为秀丽隐杆线虫的中胚层和内胚层规格的必要条件。但是,我们以前已经提供了证据,表明med-1 / 2基因的母亲表达或合子表达都不是确定秀丽隐杆线虫内胚层的必要条件。与我们的结论相反,最近的一份报告基于推测的转基因诱导的共抑制作用提供了证据,证明med-1 / 2基因确实显示出内胚层特异性母体效应。在本文中,我们对med-2(-)进行了重新研究; med-1(-)胚胎使用med-2特异性无效等位基因代替以前使用的染色体缺陷,并证实了我们先前的结果:med-2(-)的绝大多数(约84%); med-1(-)胚胎表达肠道颗粒。我们还使用已知有效消灭母本转录本的标准方案,将med dsRNA直接注射入致敏(缺药)的雌雄同体中,再次研究了母本med-1 / 2效应的可能性,但再次没有发现任何显着的母本证据med-1 / 2效果。但是,我们确实表明,在med-1 / 2缺陷型胚胎中肠道颗粒的表达对液泡ATPase编码的unc-32基因[存在于同一多拷贝med-1(+)含转基因中)对RNAi非常敏感平衡剂用于支持孕产妇med-1 / 2效应]。因此,我们建议应重新检查母亲med-1 / 2效应的实验证据,并应反映由多个转基因unc-32序列而非med序列引起的共抑制。

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