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内体中不存在鞘磷脂合酶。

Sphingomyelin synthase is absent from endosomes.

作者信息

van Helvoort A, Stoorvogel W, van Meer G, Burger N J

机构信息

Department of Cell Biology, Faculty of Medicine and Institute of Biomembranes, Universiteit Utrecht, The Netherlands.

出版信息

J Cell Sci. 1997 Mar;110 ( Pt 6):781-8. doi: 10.1242/jcs.110.6.781.

DOI:10.1242/jcs.110.6.781
PMID:9099952
Abstract

Both the Golgi and the endosomes have recently been proposed as the main site of SM-synthase, the enzyme responsible for sphingomyelin (SM) biosynthesis. To settle this confusion, we studied the subcellular distribution of SM-synthase in human liver-derived HepG2 and baby hamster kidney BHK-21 cells. To discriminate between Golgi and endosomes we made use of 3,3-diaminobenzidine (DAB) cytochemistry. Cells were incubated with a conjugate of transferrin (Tf) and horseradish peroxidase (HRP), or with unconjugated HRP, to label the recycling pathway and the complete endocytic pathway (including lysosomes) with peroxidase activity, respectively. After cell homogenization, the peroxidase activity was used to induce a local deposition of DAB-polymer. The total SM-synthase activity was not affected by this procedure, and, in contrast to endosomes labeled with (125)I-Tf, organelles containing SM-synthase did not increase in buoyant density as determined by Percoll density gradient fractionation. Thus, little, if any, SM-synthase localizes to the endocytic pathway of HepG2 and BHK-21 cells. In experiments performed at low temperature to inhibit vesicular transport, we found less than 10% of newly synthesized short-chain SM at the cell surface. We conclude that most SM-synthase activity is present in the Golgi, and to a small extent at the cell surface.

摘要

最近有人提出,高尔基体和内体都是鞘磷脂合酶的主要位点,该酶负责鞘磷脂(SM)的生物合成。为了解决这一争议,我们研究了鞘磷脂合酶在人肝脏来源的HepG2细胞和幼仓鼠肾BHK - 21细胞中的亚细胞分布。为了区分高尔基体和内体,我们利用了3,3 - 二氨基联苯胺(DAB)细胞化学技术。分别用转铁蛋白(Tf)与辣根过氧化物酶(HRP)的偶联物或未偶联的HRP孵育细胞,以分别标记具有过氧化物酶活性的再循环途径和完整的内吞途径(包括溶酶体)。细胞匀浆后,利用过氧化物酶活性诱导DAB聚合物的局部沉积。该过程不影响总的鞘磷脂合酶活性,并且与用(125)I - Tf标记的内体相反,通过Percoll密度梯度分级分离测定,含有鞘磷脂合酶的细胞器的浮力密度并未增加。因此,HepG2和BHK - 21细胞的内吞途径中几乎没有鞘磷脂合酶(如果有的话)。在低温下进行的抑制囊泡运输的实验中,我们发现在细胞表面新合成的短链SM不到10%。我们得出结论,大多数鞘磷脂合酶活性存在于高尔基体中,在细胞表面有少量存在。

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