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HeLa细胞中显微注射蛋白质自噬的证据。

Evidence for the autophagy of microinjected proteins in HeLA cells.

作者信息

Stacey D W, Allfrey V G

出版信息

J Cell Biol. 1977 Dec;75(3):807-17. doi: 10.1083/jcb.75.3.807.

Abstract

Rhodamine-conjugated proteins were microinjected into living HeLa cells. Fluorescence microscopy was then employed to study their segregation from the cytoplasm into lysosomes. Results obtained in this way were verified when the corresponding unconjugated proteins were localized by autoradiographic, histological, and antibody-staining methods after their microinjection. Most injected proteins were segregated into cytoplasmic granular structures during their removal from cells. As evidence that these were autophagic vacuoles, they were found to contain no detectable acid phosphatase activity upon formation, after which they moved to the juxtanuclear position of lysosomes and appeared to fuse with them. The segregation of microinjected proteins exhibited a high degree of selectivity. The half-times of placement of individual exogenous proteins into cytoplasmic granules varied from 3 h to nearly 3 days, and one protein, hemoglobin, was never observed to enter them. Furthermore, endogenous HeLa proteins in a size fraction near 200,000 daltons were segregated much more rapidly than those in a fraction near 40,000 daltons. In these studies, rapid protein segregation appeared to take place by a mechanism of exclusion of the injected protein from numerous cytoplasmic domains.

摘要

将罗丹明偶联的蛋白质显微注射到活的HeLa细胞中。然后利用荧光显微镜研究它们从细胞质向溶酶体的分离。当通过放射自显影、组织学和抗体染色方法对相应的未偶联蛋白质进行显微注射后的定位时,以这种方式获得的结果得到了验证。大多数注射的蛋白质在从细胞中清除的过程中被分离到细胞质颗粒结构中。作为这些是自噬泡的证据,发现它们在形成时不含有可检测到的酸性磷酸酶活性,之后它们移动到溶酶体的核旁位置并似乎与它们融合。显微注射蛋白质的分离表现出高度的选择性。将单个外源蛋白质放置到细胞质颗粒中的半衰期从3小时到近3天不等,并且从未观察到一种蛋白质血红蛋白进入它们。此外,分子量接近200,000道尔顿的HeLa内源蛋白质的分离比分子量接近40,000道尔顿的部分中的蛋白质快得多。在这些研究中,快速的蛋白质分离似乎是通过将注射的蛋白质从许多细胞质区域中排除的机制发生的。

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