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一种方蟹科螃蟹中用于光感受器膜降解的酸性水解酶来源。

The sources of acid hydrolases for photoreceptor membrane degradation in a grapsid crab.

作者信息

Blest A D, Stowe S, Price D G

出版信息

Cell Tissue Res. 1980;205(2):229-44. doi: 10.1007/BF00234682.

DOI:10.1007/BF00234682
PMID:7357573
Abstract

Dawn photoreceptor breakdown in the crab Leptograpsus variegatus is analysed at the ultrastructural level. Coated vesicles derived from microvilli are assembled as mutlivesicular bodies (mvbs), which degrade to multilamellar bodies (mls) and are lysed. Cytochemical markers for hydrolases were a fluoride-inhibited beta-glycerophosphatase and a fluoride-insensitive p-nitrophenyl phosphatse, with indistinguishable distributions when localised at pH 5.0. These enzymes are injected into the secondary lysomes from two sources: (i) immediately after dawn Golgi bodies are highly active, and differentiate a transtubular network, from which tubules and vesicles detach, and can be seen fusing with mvbs and mlbs. (ii) Saccules derived from the rough endoplasmic reticulum (RER) provide a second source and are most often seen in association with late mlbs. Both kinds of primary lysosome rare give AcPh-positive responses when free in the cytosol, but are seen to do so as they make contact with their secondary lysosomal targets. Lipid droplets and lipofuscin bodies are interpreted as the residual products of breakdown. These results are discussed in relation to previous findings on photoreceptor membrane breakdown in a dinopid spider. Attention is drawn to the implied diversity of organisation of lysosomal compartments in receptors which internalise membranes of similar compositions.

摘要

在超微结构水平上分析了杂色厚蟹黎明时分光感受器的分解情况。源自微绒毛的被膜小泡组装成多囊泡体(mvbs),多囊泡体降解为多层体(mls)并被溶解。水解酶的细胞化学标记物是氟化物抑制的β-甘油磷酸酶和对氟化物不敏感的对硝基苯磷酸酶,当在pH 5.0定位时,它们的分布难以区分。这些酶从两个来源注入次级溶酶体:(i)黎明后不久,高尔基体高度活跃,并分化出一个跨管状网络,从中分离出小管和小泡,可以看到它们与多囊泡体和多层体融合。(ii)源自粗面内质网(RER)的扁平囊提供了第二个来源,最常与晚期多层体相关联。这两种初级溶酶体在胞质溶胶中游离时很少产生酸性磷酸酶阳性反应,但在与次级溶酶体靶标接触时会产生这种反应。脂滴和脂褐素体被解释为分解的残余产物。结合先前关于Dinopid蜘蛛光感受器膜分解的研究结果对这些结果进行了讨论。人们注意到,在内化相似组成膜的受体中,溶酶体区室组织的潜在多样性。

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