使用硝酸铅进行腺苷酸环化酶活性组织化学显示时的陷阱。

Pitfalls in the use of lead nitrate for the histochemical demonstration of adenylate cyclase activity.

作者信息

Lemay A, Jarett L

出版信息

J Cell Biol. 1975 Apr;65(1):39-50. doi: 10.1083/jcb.65.1.39.

DOI:10.1083/jcb.65.1.39

PMID:165205

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2111165/

Abstract

The biochemistry of the lead histochemical technique for demonstrating adenylate cyclase was studied. The enzyme activity of fat cell plasma membranes, using 5'-adenylyl-imidodiphosphate (AMP-PNP) as substrate, was completely inhibited at 1 times 10- minus 4 M Pb(NO3)2 and yet at 4 times 10- minus 3 M Pb(NO3)2 precipitate could be demonstrated by electron microscopy on both sides of plasma membrane vesicles. No lead-diphosphoimide or lead-phosphate precipitate could be visualized by electron microscopy when the lead was reduced to a level (2 times 10- minus 5 M) which caused only 50% inhibition of the enzyme. A solubility product coefficient of 1 times 10- minus 10 M was found necessary to allow precipitation of lead-phosphate complex in the adenylate cyclase medium. Varying the ratio of substrate or dextran relative to the lead failed to protect the inhibition of the enzyme. Increasing concentrations of beta-mercaptoethanol restored the basal and stimulated activity of adenylate cyclase but also prevented the precipitation reaction. Lead at 2 times 10- minus 3 M caused the nonenzymatic hydrolysis of AMP-PNP, resulting in the production of small but significant quantities of cyclic AMP and substantial amounts of AMP. This hydrolysis was inhibited by alloxan but unaffected by dextran of NaF. The adenylate cyclase activity of pancreatic islet homogenates and of fat pad capillaries was completely inhibited by lead concentrations equal to or less than those used in histochemical studies (Howell, S. L., and M. Whitfield. 1972. J. Histochem. Cytochem. 20:873-879. and Wagner, R. C., P. Kreiner, R. J. Barrnett, and M. W. Bitensky. 1972. Proc. Natl. Acad. Sci. U.S.A. 69:3175-3179.). The present study shows that the lead histochemical method cannot be used for localization of adenylate cyclase because of the inhibition of the enzyme and artifacts produced by high lead concentrations and the inability to produce a visible precipitate at low lead concentrations which only partially inhibit the enzyme.

摘要

对用于显示腺苷酸环化酶的铅组织化学技术的生物化学进行了研究。以5'-腺苷酰亚氨二磷酸（AMP-PNP）为底物时，脂肪细胞质膜的酶活性在1×10⁻⁴M硝酸铅中完全被抑制，但在4×10⁻³M硝酸铅时，通过电子显微镜可在质膜囊泡两侧显示沉淀。当铅浓度降至仅导致酶活性50%抑制的水平（2×10⁻⁵M）时，电子显微镜下未观察到铅-二磷酸亚胺或磷酸铅沉淀。发现腺苷酸环化酶培养基中磷酸铅复合物沉淀所需的溶度积系数为1×10⁻¹⁰M。改变底物或葡聚糖与铅的比例未能保护酶免受抑制。增加β-巯基乙醇的浓度可恢复腺苷酸环化酶的基础活性和刺激活性，但也可防止沉淀反应。2×10⁻³M的铅导致AMP-PNP的非酶水解，产生少量但显著量的环磷酸腺苷和大量的腺苷一磷酸。这种水解被四氧嘧啶抑制，但不受氟化钠或葡聚糖的影响。胰腺胰岛匀浆和脂肪垫毛细血管的腺苷酸环化酶活性在等于或低于组织化学研究中所用铅浓度时被完全抑制（豪厄尔，S.L.，和M.惠特菲尔德。1972年。《组织化学与细胞化学杂志》20:873 - 879。以及瓦格纳，R.C.，P.克莱纳，R.J.巴尼特，和M.W.比滕斯基。1972年。《美国国家科学院院刊》69:3175 - 3179）。本研究表明，由于酶被抑制、高铅浓度产生的假象以及在仅部分抑制酶的低铅浓度下无法产生可见沉淀，铅组织化学方法不能用于腺苷酸环化酶的定位。