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酸性磷酸酶的细胞化学与生物化学。III. 大鼠腹侧前列腺溶酶体和分泌性酸性磷酸酶的抑制实验。

Cytochemistry and biochemistry of acid phosphatases. III. Inhibition experiments of lysosomal and secretory acid phosphatases of the rat ventral prostate.

作者信息

Seitz J, Aumuller G

出版信息

Basic Appl Histochem. 1981;25(2):95-104.

PMID:6455992
Abstract

Biochemical and cytochemical inhibition experiments of rat prostatic acid phosphatase were performed using enzymes separated on isoelectric focusing (IEF) gels, and thin sections of the rat ventral prostate. Various inhibitors, including L (+) tartrate, mercuric ions and sodium fluoride were applied to electrofocused enzymes which were subsequently stained for acid phosphatase activity. Enzymes focused on IEF gels at pH 7.9 and 8.1, respectively, were inhibited with 1.8 x 10-3 M tartrate, while the enzyme activities with isoelectric points (pl) of 5.6 and 7.15, respectively, were only slightly inhibited by this compound. Using 10-3M mercuric ions, enzymes with pl of 5.6 and 7.15 were inhibited while the enzymes with pl of 7.9 and 8.1 were still active. The biochemical procedures were adapted to chopper sections of perfused-fixed ventral prostate of the rat. Preincubation of the sections with 2.4 x 10-3M mercuric chloride blocked the secretory enzyme and most of the lysosomal enzyme and resulted in an artificial staining of the Golgi apparatus and other cytoplasmic organelles. Nuclear precipitates however were prevented. L (+) tartrate could not be used at the ultrastructural level since it developed false positive results by the formation of lead tartrate. The results indicate that no selective inhibition of either secretory or lysosomal acid phosphatase can be achieved at the ultrastructural level using metal salts or tartrate, respectively.

摘要

利用在等电聚焦(IEF)凝胶上分离出的酶以及大鼠腹侧前列腺的薄切片,对大鼠前列腺酸性磷酸酶进行了生化和细胞化学抑制实验。将包括L(+)酒石酸盐、汞离子和氟化钠在内的各种抑制剂应用于经电聚焦的酶,随后对这些酶进行酸性磷酸酶活性染色。分别聚焦于pH 7.9和8.1的IEF凝胶上的酶,用1.8×10⁻³M酒石酸盐抑制,而等电点(pI)分别为5.6和7.15的酶活性仅受到该化合物的轻微抑制。使用10⁻³M汞离子时,pI为5.6和7.15的酶受到抑制,而pI为7.9和8.1的酶仍具有活性。生化程序适用于灌注固定的大鼠腹侧前列腺的切片。用2.4×10⁻³M氯化汞对切片进行预孵育,可阻断分泌酶和大部分溶酶体酶,并导致高尔基体和其他细胞质细胞器的人工染色。然而,可防止核沉淀物的产生。由于L(+)酒石酸盐会因形成酒石酸铅而产生假阳性结果,因此不能在超微结构水平上使用。结果表明,分别使用金属盐或酒石酸盐在超微结构水平上无法实现对分泌性或溶酶体酸性磷酸酶的选择性抑制。

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