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大肠杆菌核糖体蛋白S15编码mRNA的衰变由核糖核酸酶E依赖性内切核酸酶切割引发,该切割去除了3'稳定茎环结构。

Decay of mRNA encoding ribosomal protein S15 of Escherichia coli is initiated by an RNase E-dependent endonucleolytic cleavage that removes the 3' stabilizing stem and loop structure.

作者信息

Régnier P, Hajnsdorf E

机构信息

Institut de Biologie Physico Chimique, Paris, France.

出版信息

J Mol Biol. 1991 Jan 20;217(2):283-92. doi: 10.1016/0022-2836(91)90542-e.

Abstract

The transcripts of the rpsO-pnp operon of Escherichia coli, coding for ribosomal protein S15 and polynucleotide phosphorylase, are processed at four sites in the 249 nucleotides of the intercistronic region. The initial processing step in the decay of the pnp mRNA is made by RNase III, which cuts at two sites upstream from the pnp gene. The other two cleavages are dependent on the wild-type allele of the rne gene, which encodes the endonucleolytic enzyme RNase E. The cuts are made 37 nucleotides apart at the base of the stem-loop structure of the rho-independent attenuator located downstream from rpsO. The cleavage downstream from the attenuator generates an rpsO mRNA.nearly identical with the monocistronic attenuated transcript, while the cleavage upstream from the transcription attenuator gives rise to an rpsO mesage lacking the terminal 3' hairpin structure. The rapid degradation of the processed mRNA in an rne+ strain, compared to the slow degradation of the transcript that accumulates in an rne- strain, suggests that RNase E initiates the decay of the rpsO message by removing the stabilizing stem-loop at the 3' end of the RNA.

摘要

大肠杆菌的rpsO-pnp操纵子转录本编码核糖体蛋白S15和多核苷酸磷酸化酶,在基因间区域的249个核苷酸中的四个位点进行加工。pnp mRNA降解的初始加工步骤由RNase III完成,它在pnp基因上游的两个位点切割。另外两个切割依赖于rne基因的野生型等位基因,该基因编码内切核酸酶RNase E。切割在位于rpsO下游的不依赖ρ因子的衰减子的茎环结构底部相隔37个核苷酸处进行。衰减子下游的切割产生一个与单顺反子衰减转录本几乎相同的rpsO mRNA,而转录衰减子上游的切割产生一个缺少末端3'发夹结构的rpsO信息。与rne-菌株中积累的转录本缓慢降解相比,rne+菌株中加工后的mRNA快速降解,这表明RNase E通过去除RNA 3'端的稳定茎环结构来启动rpsO信息的降解。

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