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包膜病毒粒子(水疱性口炎病毒)膜结构的13C-核磁共振研究

13C-NMR studies of the membrane structure of enveloped virions (vesicular stomatitis virus).

作者信息

Stoffel W, Bister K, Schreiber C, Tunggal B

出版信息

Hoppe Seylers Z Physiol Chem. 1976 Jul;357(7):905-15. doi: 10.1515/bchm2.1976.357.2.905.

Abstract

The mobility of the lipids in the bilayer of the envelope of vesicular stomatitis virus has been probed over its complete space by the biosynthetic incorporation of [N-13CH3]- choline as a probe for the polar head groups and [3-13C]- and [11-13C] oleic acid and [16-13C]- palmitic acid for the hydrophobic region of the bilayer. These precursors were effectively incorporated as established by the concomitant administration of the same precursors in radioactive form. Spin lattice relaxation time measurements (T1) of the 13C enriched segments in complete virus envelope allowed estimation of their mobility. The mobility of the polar head groups is restricted, probably due to ionic interactions with neighbouring acidic phospholipids (phosphatidylserine) and/or acidic side chains of the glycoprotein (G-protein). The rigidity of the hydrophobic part of the bilayer is due to the high cholesterol content and interaction with the immersing polypeptide chains of the G- and possibly M-protein. The rigidity is limited to a depth of about 15 A ranging from the inner and outer surface, whereas the inner core of the bilayer is fluid. Tryptic cleavage of the hydrophilic part of the G-protein allows the lipophilic immersing polypeptide fragment to enter further the bilayer which then reduces the fluidity of the hydrocarbon chains in the core region by lipid-protein interactions.

摘要

通过生物合成掺入[ N - 13CH3 ] - 胆碱作为极性头部基团的探针,以及[ 3 - 13C ] - 、[ 11 - 13C ] - 油酸和[ 16 - 13C ] - 棕榈酸作为双层疏水区域的探针,对水疱性口炎病毒包膜双层中脂质的流动性在其整个空间进行了探测。通过同时给予相同放射性形式的前体证实,这些前体被有效地掺入。对完整病毒包膜中13C富集片段的自旋晶格弛豫时间测量(T1),使得能够估计它们的流动性。极性头部基团的流动性受到限制,这可能是由于与相邻酸性磷脂(磷脂酰丝氨酸)和/或糖蛋白(G蛋白)的酸性侧链发生离子相互作用所致。双层疏水部分的刚性归因于高胆固醇含量以及与G蛋白和可能的M蛋白的浸入多肽链的相互作用。这种刚性限制在从内表面和外表面起约15埃的深度范围内,而双层的内核是流体状的。对G蛋白亲水部分进行胰蛋白酶切割,使得亲脂性浸入多肽片段能够进一步进入双层,然后通过脂质 - 蛋白质相互作用降低核心区域烃链的流动性。

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