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通过诱变确定酵母RNA聚合酶II(B)活性位点中亲和标记的赖氨酸残基

Determination of lysine residues affinity labeled in the active site of yeast RNA polymerase II(B) by mutagenesis.

作者信息

Treich I, Carles C, Sentenac A, Riva M

机构信息

Service de Biochimie et Génétique Moléculaire, Centre d'Etudes de Saclay, Gif sur Yvette, France.

出版信息

Nucleic Acids Res. 1992 Sep 25;20(18):4721-5. doi: 10.1093/nar/20.18.4721.

Abstract

In a previous study, yeast RNA polymerase II(B) was affinity labeled with two nucleotide derivatives (III and VIII) (1). In both cases, the labeled site was localized to the C-terminal part of the B150 subunit. The potential target lysyl residues of derivative III were mapped to the conserved domain H, between Asn946 and Met999. In the present work, we have mutagenized to arginine the five lysines present in domain H. Three lysines can be replaced, individually or simultaneously, without affecting cell growth, and each mutated enzyme can still be affinity labeled. Hence one or both of the other two lysyl residues, Lys979 and Lys987, is the target of the affinity reagent. These two lysines were each found to be essential for cell viability. Derivative VIII labeled another domain in addition to domain H. Supported by analogous results obtained for E. coli RNA polymerase using derivative VIII (2), we hypothesized that the second domain labeled by this derivative in the B150 subunit was domain I. Mutagenesis of the unique lysine present in domain I demonstrated that Lys 1102 was the target of derivative VIII. These results indicate that in both prokaryotic and eukaryotic RNA polymerases, domains H and I are in close proximity and participate to the active site.

摘要

在先前的一项研究中,酵母RNA聚合酶II(B) 用两种核苷酸衍生物(III和VIII)进行了亲和标记(1)。在这两种情况下,标记位点都定位于B150亚基的C末端部分。衍生物III的潜在靶赖氨酸残基被定位到Asn946和Met999之间的保守结构域H。在本研究中,我们将结构域H中存在的五个赖氨酸突变为精氨酸。三个赖氨酸可以单独或同时被取代,而不影响细胞生长,并且每种突变酶仍然可以被亲和标记。因此,另外两个赖氨酸残基Lys979和Lys987中的一个或两个是亲和试剂的靶标。发现这两个赖氨酸对于细胞活力都是必不可少的。衍生物VIII除了标记结构域H外,还标记了另一个结构域。基于使用衍生物VIII对大肠杆菌RNA聚合酶获得的类似结果的支持(2),我们推测该衍生物在B150亚基中标记的第二个结构域是结构域I。对结构域I中存在的唯一赖氨酸进行诱变表明,Lys 1102是衍生物VIII的靶标。这些结果表明,在原核和真核RNA聚合酶中,结构域H和I都紧密相邻并参与活性位点的构成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c5be/334223/680c926f7a29/nar00229-0033-a.jpg

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