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禽逆转录病毒pp12蛋白与病毒RNA相互作用的特征及调控

Characteristics and regulation of interaction of avian retrovirus pp12 protein with viral RNA.

作者信息

Leis J, Jentoft J

出版信息

J Virol. 1983 Nov;48(2):361-9. doi: 10.1128/JVI.48.2.361-369.1983.

DOI:10.1128/JVI.48.2.361-369.1983
PMID:6312093
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC255360/
Abstract

We investigated the interaction of the avian retrovirus pp12 protein with viral RNA to assess its possible role in virion assembly. Using chemical modification techniques, we found that reagents specific for lysine or arginine residues inactivated the RNA-binding capacity of the protein. The binding of pp12 to 60S viral RNA was also strongly affected by pH (pKapp of 5.5); the affinity for viral RNA decreased by as much as 40-fold after protonation of one or more titratable groups on the protein. When the protein was cleaved by cyanogen bromide, each of the two polypeptide products bound to RNA (with low affinity), but pH dependence was lost. Thus, an intact protein was required for this effect. Since histidine and phosphoserine residues have pKa values close to the pKapp of the pp12-RNA interaction, they were studied to determine whether they were involved in this process. Each of the two histidyl residues in pp12 had pKa values of 6.2, as determined by proton nuclear magnetic resonance titrations, values too high to account for the pKapp of binding. The involvement of phosphoserine residues, which have pKa values similar to the pKapp, was investigated by removal of phosphate from pp12. When phosphate groups were chemically or enzymatically removed from the avian myeloblastosis virus, Rous sarcoma virus (Pr-C), and PR-E 95C virus pp12 proteins, the Kapp for binding 60S viral RNA was reduced 100-fold at pH 7.5. Thus, it seems possible that phosphorylation of the pp12 protein could favor viral nucleocapsid formation by increasing its affinity for the viral RNA genome. Dephosphorylation could provide for its release from the viral RNA during reverse transcription after viral infection of cells.

摘要

我们研究了禽逆转录病毒pp12蛋白与病毒RNA的相互作用,以评估其在病毒粒子组装中可能发挥的作用。使用化学修饰技术,我们发现针对赖氨酸或精氨酸残基的试剂会使该蛋白的RNA结合能力失活。pp12与60S病毒RNA的结合也受到pH值(表观解离常数pKapp为5.5)的强烈影响;蛋白质上一个或多个可滴定基团质子化后,对病毒RNA的亲和力下降了多达40倍。当该蛋白被溴化氰切割时,两个多肽产物均与RNA结合(亲和力较低),但失去了pH依赖性。因此,这种效应需要完整的蛋白。由于组氨酸和磷酸丝氨酸残基的pKa值接近pp12-RNA相互作用的pKapp,因此对它们进行了研究,以确定它们是否参与这一过程。通过质子核磁共振滴定法测定,pp12中的两个组氨酸残基的pKa值均为6.2,该值过高,无法解释结合的pKapp。通过去除pp12中的磷酸基团,研究了磷酸丝氨酸残基(其pKa值与pKapp相似)的参与情况。当从禽成髓细胞瘤病毒、劳氏肉瘤病毒(Pr-C)和PR-E 95C病毒的pp12蛋白中化学或酶法去除磷酸基团时,在pH 7.5条件下,与60S病毒RNA结合的表观解离常数Kapp降低了100倍。因此,pp12蛋白的磷酸化似乎有可能通过增加其对病毒RNA基因组的亲和力来促进病毒核衣壳的形成。去磷酸化则可以使其在病毒感染细胞后逆转录过程中从病毒RNA上释放出来。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3d41/255360/7f2c6ea7c013/jvirol00140-0039-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3d41/255360/7f2c6ea7c013/jvirol00140-0039-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3d41/255360/7f2c6ea7c013/jvirol00140-0039-a.jpg

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