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通过一种内在光亲和探针获得的大肠杆菌30S核糖体亚基1和2结构域中的新型RNA-蛋白质交联。

New RNA-protein crosslinks in domains 1 and 2 of E. coli 30S ribosomal subunits obtained by means of an intrinsic photoaffinity probe.

作者信息

Hajnsdorf E, Favre A, Expert-Bezançon A

机构信息

Institut Jacques Monod, CNRS-Université Paris VII, France.

出版信息

Nucleic Acids Res. 1989 Feb 25;17(4):1475-91. doi: 10.1093/nar/17.4.1475.

Abstract

Functionally active 70S ribosomes containing 4-thiouridine (s4U) in place of uridine were prepared by a formerly described in vivo substitution method. Proteins were crosslinked to RNA by 366 nm photoactivation of s4U. We observe the systematic and characteristic formation of 30S dimers; they were eliminated for analysis of RNA-protein crosslinks. M13 probes containing rDNA inserts complementary to domains 1 and 2 of 16S RNA from the 5'end up to nucleotide 868 were used to select contiguous or overlapping RNA sections. The proteins covalently crosslinked to each RNA section were identified as S3, S4, S5, S7, S9, S18, S20 and S21. Several crosslinks are compatible with previously published sites for proteins S5, S18, S20 and S21; others for proteins S3, S4, S7, S9, S18 correspond necessarily to new sites.

摘要

通过先前描述的体内置换方法制备了功能活性的70S核糖体,其中用4-硫尿苷(s4U)取代了尿苷。通过s4U的366nm光活化使蛋白质与RNA交联。我们观察到30S二聚体的系统性和特征性形成;为了分析RNA-蛋白质交联,将它们去除。含有与16S RNA 5'端至核苷酸868的结构域1和2互补的rDNA插入片段的M13探针用于选择连续或重叠的RNA片段。与每个RNA片段共价交联的蛋白质被鉴定为S3、S4、S5、S7、S9、S18、S20和S21。几个交联与先前发表的蛋白质S5、S18、S20和S21的位点相符;其他与蛋白质S3、S4、S7、S9、S18的交联必然对应于新位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/988f/331816/b3f5709314d0/nar00213-0207-a.jpg

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