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cDNA cloning confirms the polyadenylation of RNA decay intermediates in Streptomyces coelicolor

机译:cDNA克隆证实RNA衰减中间体在链霉菌中的中间体的聚酰基化

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In Escherichia coli the poly(A) tails of messenger and rRNAs are a major determinant of RNA stability. These tails are formed primarily by poly(A) polymerase I (PAP I) in wild-type strains or by polynucleotide phosphorylase (PNPase) in PAP I-deficient strains. In Streptomyces coelicolor it has been shown that mycelial RNAs display biochemical characteristics consistent with the presence of poly(A) tails. To confirm the occurrence of polyadenylation, rRNA and mRNA transcripts from S. coelicolor were isolated by oligo(dT)-dependent RT-PCR followed by cDNA cloning. One of the clones obtained was polyadenylated at a site corresponding to the mature 3′ terminus of 16S rRNA, while two 23S rRNA cDNA clones were polyadenylated at precursor processing sites. Other clones identified polyadenylation sites internal to the coding regions of both 16S and 23S rRNAs, and redD and actII-orf4 mRNAs. While most rRNA cDNA clones displayed adenosine homopolymer tails, the poly(A) tails of three rRNAs and all the redD and actII-orf4 clones consisted of a variety of heteropolymers. These results suggest that the enzyme primarily responsible for polyadenylation in S. coelicolor is PNPase rather than a PAP I homologue.
机译:在大肠杆菌中,Messenger和RRNA的Poly(a)尾部是RNA稳定性的主要决定因素。这些尾部主要由野生型菌株的聚(A)聚合酶I(PAP I)或PAP I缺陷菌株中的多核苷酸磷酸化酶(PNPase)形成。在链霉菌中的菌胶质溶胶中,已经表明,菌丝体RNA显示与聚(a)尾部的存在一致的生物化学特性。为了确认从寡核苷酸(DT) - 依赖性RT-PCR中分离来自S.的rRNA和MRNA转录物的rRNA和mRNA转录物,然后通过cDNA克隆。在对应于16S rRNA的成熟3'末端的位点处得到的其中一种克隆在对应于16S rRNA的成熟3'末端,而在前体加工位点是聚腺苷酸化的两种23s rRNA cDNA克隆。其他克隆鉴定了16S和23S RRNA的编码区域内的多腺苷酸化位点,以及REDD和ACTII-ORF4 mRNA。虽然大多数RRNA cDNA克隆显示腺苷均聚物尾,但三个RRNA的聚(a)尾部和所有的REDD和ACTII-ORF4克隆组成,包括各种杂聚物。这些结果表明,酶主要负责在S.共苯基中的多腺苷酸化是PNPase而不是PAP I同源物。

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