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II型肺细胞中板层小体与溶酶体的关系。

The relationship between lamellar bodies and lysosomes in type II pneumocytes.

作者信息

Gibson K F, Widnell C C

机构信息

Department of Neurobiology, University of Pittsburgh, School of Medicine, Pennsylvania 15261.

出版信息

Am J Respir Cell Mol Biol. 1991 Jun;4(6):504-13. doi: 10.1165/ajrcmb/4.6.504.

Abstract

We have studied the relationship between lysosomes and lamellar bodies in alveolar type II (ATII) pneumocytes using a monoclonal antibody (anti-lgp-120) directed against a 120-kD rat lysosomal membrane glycoprotein and a polyclonal antibody (anti-SP-A) directed against rat surfactant protein A. The anti-lgp-120 precipitated a protein molecular mass of 120 kD from Triton cell lysates radiolabeled with [35S]methionine, and the anti-SP-A precipitated surfactant apoprotein A from the medium when analyzed under similar conditions. When ATII cells were cultured on Engelbreth-Holm-Swarm tumor basement membrane, and studied by indirect immunofluorescence, some structures seem to react with both antibodies, and others with only one. ATII cells cultured on plastic showed a major population of large vesicles that were labeled intensely with both antibodies, and a second population of vesicles that were labeled weakly and only with anti-SP-A. Analytical cell fractionation of freshly isolated ATII cells confirmed that lgp-120 was only present in structures containing the lysosomal matrix enzyme N-acetyl-beta-glucosaminidase. In contrast, SP-A was identified in two populations of vesicles with high phospholipid-to-protein ratios: one lacked N-acetyl-beta-glucosaminidase and lgp-120 and contained lamellar bodies; the other contained both lysosomal markers and a heterogeneous population of organelles that included multivesicular bodies, lamellar bodies, and lysosomes. Western blots of trichloroacetic acid precipitates of cell fractions identified proteins within the lysosomal compartment that reacted with anti-SP-A, but whose molecular mass was less than 28 kD. The results indicate that, in ATII cells, surfactant is located in two functionally distinct structures, one of which is probably involved in surfactant secretion, and the other, surfactant degradation. The techniques developed in this study should allow the role of these structures in the secretion and recycling of surfactant to be determined.

摘要

我们使用针对120-kD大鼠溶酶体膜糖蛋白的单克隆抗体(抗lgp-120)和针对大鼠表面活性蛋白A的多克隆抗体(抗SP-A),研究了肺泡II型(ATII)肺细胞中溶酶体与板层小体之间的关系。抗lgp-120从用[35S]甲硫氨酸进行放射性标记的Triton细胞裂解物中沉淀出分子量为120 kD的蛋白质,在相似条件下分析时,抗SP-A从培养基中沉淀出表面活性载脂蛋白A。当ATII细胞在Engelbreth-Holm-Swarm肿瘤基底膜上培养并用间接免疫荧光法研究时,一些结构似乎与两种抗体都发生反应,而另一些则只与一种抗体反应。在塑料上培养的ATII细胞显示出主要的一大群大囊泡,两种抗体都对其进行了强烈标记,还有第二群囊泡,标记较弱,且仅被抗SP-A标记。对新鲜分离的ATII细胞进行分析性细胞分级分离证实,lgp-120仅存在于含有溶酶体基质酶N-乙酰-β-葡萄糖胺酶的结构中。相反,在两群具有高磷脂与蛋白质比率的囊泡中鉴定出了SP-A:一群缺乏N-乙酰-β-葡萄糖胺酶和lgp-120,含有板层小体;另一群既含有溶酶体标记物,又含有包括多囊泡体、板层小体和溶酶体在内的异质性细胞器群体。细胞分级分离物的三氯乙酸沉淀物的蛋白质免疫印迹法鉴定出溶酶体区室内与抗SP-A反应但其分子量小于28 kD的蛋白质。结果表明,在ATII细胞中,表面活性物质位于两个功能不同的结构中,其中一个可能参与表面活性物质的分泌,另一个则参与表面活性物质的降解。本研究中开发的技术应能确定这些结构在表面活性物质的分泌和再循环中的作用。

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