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球形红假单胞菌胞质内膜系统的拓扑结构与生长:蛋白质、叶绿素和磷脂插入稳态厌氧细胞的过程

Topology and growth of the intracytoplasmic membrane system of Rhodopseudomonas spheroides: protein, chlorophyll, and phospholipid insertion into steady-state anaerobic cells.

作者信息

Kosakowski M H, Kaplan S

出版信息

J Bacteriol. 1974 Jun;118(3):1144-57. doi: 10.1128/jb.118.3.1144-1157.1974.

DOI:10.1128/jb.118.3.1144-1157.1974
PMID:4545399
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC246865/
Abstract

An equilibrium density gradient centrifugation study involving the separation of "old" and "new" membranes has been developed to determine the manner in which protein, lipid, and chlorophyll are incorporated into growing intracytoplasmic membranes (chromatophores) of Rhodopseudomonas spheroides. Chromatophores derived from cells grown in an H(2)O-medium had a density of 1.175 to 1.180 g/cm(3) and were readily separable from chromatophores having a density of 1.220 to 1.230 isolated from cells grown in a 70% D(2)O-medium. After a shift from "D(2)O-" to "H(2)O"-based media, only hybrid chromatophores derived from a combination of "heavy" (old) and "light" (new) chromatophore material could be detected. The experimentally determined, median density values for the growing intracytoplasmic membrane system followed a theoretically determined profile which was calculated from the density of full "heavy" and full "light" material assuming random, homogeneous incorporation of new material into old membrane. The distribution of the radioactive labels for protein (leucine) and chlorophyll (delta-aminolevulinic acid) were identical and showed a reproducible displacement of the "old" material to the heavy side of the optical density at 365 nm (OD(365)) absorbance and a displacement of the "new" material to the light side of the OD(365) absorbance profile. Specific phospholipid growth showed no displacement for either the "old" or "new" material from the median absorbance profile.

摘要

已开展一项平衡密度梯度离心研究,该研究涉及“旧”膜和“新”膜的分离,以确定蛋白质、脂质和叶绿素掺入球形红假单胞菌生长中的胞内膜(载色体)的方式。来自在H₂O培养基中生长的细胞的载色体密度为1.175至1.180 g/cm³,并且很容易与从在70% D₂O培养基中生长的细胞分离出的密度为1.220至1.230的载色体区分开来。从基于“D₂O”的培养基转变为基于“H₂O”的培养基后,只能检测到源自“重”(旧)和“轻”(新)载色体物质组合的杂交载色体。对于生长中的胞内膜系统,实验测定的中值密度值遵循理论计算得出的曲线,该曲线是根据完全“重”和完全“轻”物质的密度计算得出的,假设新物质随机、均匀地掺入旧膜中。蛋白质(亮氨酸)和叶绿素(δ-氨基乙酰丙酸)的放射性标记分布相同,并且在365 nm光密度(OD₃₆₅)吸光度下,“旧”物质可重现地向重侧位移,“新”物质向OD₃₆₅吸光度曲线的轻侧位移。特定磷脂的生长在中值吸光度曲线中,“旧”或“新”物质均未出现位移。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d7b/246865/b53656686665/jbacter00342-0394-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d7b/246865/b53656686665/jbacter00342-0394-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d7b/246865/b53656686665/jbacter00342-0394-a.jpg

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