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Simple, directional cDNA cloning for in situ transcript hybridization screens

机译:简单,定向的cDNA克隆,用于原位转录本杂交筛选

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摘要

Here, we describe a suppression PCR-based method for directional cloning of randomly primed cDNAs from small quantities of tissue. Synthesis of the first cDNA strand is conducted on oligonucleotide-coated magnetic beads. Synthesis of the second strand is accomplished using nonspecifically primed suppression PCR. This method is used to synthesize a cDNA library from zebrafish embryos at 6-9 It after fertilization. The sequencing of the clones and their use in an in situ hybridization screen to detect restricted patterns of gene transcription in zebrafish embryos showed that this method allows the rapid identification of genes that are important for development and genes that are expressed at levels undetectable by whole-mount in situ transcript hybridization. The random priming of cDNA alleviates the problems encountered in the identification of zebrafish genes from poly(dT)-primed cDNA clones caused by the long 3' UTRs frequently found in transcripts from, this organism.
机译:在这里,我们描述了一种基于抑制PCR的方法,用于从少量组织中定向克隆随机引发的cDNA。第一条cDNA链的合成在寡核苷酸包被的磁珠上进行。第二链的合成使用非特异性引发的抑制PCR完成。受精后,该方法用于从斑马鱼胚胎的6-9 It合成cDNA文库。克隆的测序及其在原位杂交筛选中用于检测斑马鱼胚胎中基因转录的受限模式的结果表明,该方法可以快速鉴定对发育至关重要的基因和表达水平,而这些水平的表达水平是整个动物无法检测到的。进行原位转录本杂交。 cDNA的随机引发减轻了在从聚(dT)引发的cDNA克隆中鉴定斑马鱼基因时遇到的问题,该问题是由这种生物的转录本中常见的长3'UTR引起的。

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