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一种用于检测人培养成纤维细胞中芳基硫酸酯酶A活性的特异性超微结构染色法。

A specific ultrastructural stain for arylsulfatase A activity in human cultured fibroblasts.

作者信息

Chang P L, Moudgil G

出版信息

J Histochem Cytochem. 1984 Jun;32(6):617-24. doi: 10.1177/32.6.6202736.

Abstract

A staining reaction was developed to specifically detect arylsulfatase A activity in the presence of arylsulfatases B and C. Nitrocatechol, generated by all arylsulfatases from the substrate p-nitrocatechol sulfate, can be coupled to produce Hatchett 's brown which reacts with 3,3'-diaminobenzidine to yield an osmiophilic polymer visible under the electron microscope. The reaction was made specific for arylsulfatase A by inhibiting arylsulfatase C activity with low pH and arylsulfatase B activity with pyrophosphate. The specificity was confirmed both by electrophoretic analysis and by patient fibroblasts deficient only in arylsulfatase A activity. Under optimal conditions for preserving structural integrity and enzyme activity, enzyme reaction deposits were found mainly around vesicles. Some of these vesicles were large and heterogeneous (48-330 nm in diameter), distributed randomly within the cytoplasm, but most of the positive-reacting vesicles were uniform in size (86 +/- 18 nm in diameter) and distributed in a peripheral zone about 0.1-0.5 micron wide. These periplasmic vesicles might be partly fused with each other or with the plasma membrane. In conclusion, a specific stain for arylsulfatase A activity suitable for light and electron microscopy and the optimal conditions for structural and enzymatic preservations were developed. Although this enzyme has been considered to be lysosomal in origin, most of the activity was detected in periplasmic vesicles near the cell surface.

摘要

开发了一种染色反应,用于在芳基硫酸酯酶B和C存在的情况下特异性检测芳基硫酸酯酶A的活性。所有芳基硫酸酯酶从底物对硝基儿茶酚硫酸酯生成的硝基儿茶酚,可以偶联生成哈奇特棕,其与3,3'-二氨基联苯胺反应,产生在电子显微镜下可见的嗜锇聚合物。通过用低pH抑制芳基硫酸酯酶C的活性和用焦磷酸盐抑制芳基硫酸酯酶B的活性,使该反应对芳基硫酸酯酶A具有特异性。通过电泳分析和仅缺乏芳基硫酸酯酶A活性的患者成纤维细胞证实了特异性。在保持结构完整性和酶活性的最佳条件下,发现酶反应沉积物主要围绕囊泡。其中一些囊泡较大且不均一(直径48 - 330 nm),随机分布在细胞质中,但大多数阳性反应囊泡大小均匀(直径86±18 nm),分布在约0.1 - 0.5微米宽的外周区域。这些周质囊泡可能彼此部分融合或与质膜融合。总之,开发了一种适用于光学和电子显微镜的芳基硫酸酯酶A活性的特异性染色方法以及结构和酶保存的最佳条件。尽管这种酶被认为起源于溶酶体,但大部分活性是在细胞表面附近的周质囊泡中检测到的。

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