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Literature DB >> 165205

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

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.

Entities: Chemical Gene

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Year: 1975 PMID： 165205 PMCID： PMC2111165 DOI： 10.1083/jcb.65.1.39

Source DB: PubMed Journal: J Cell Biol ISSN： 0021-9525 Impact factor: 10.539

23 in total

1. Histochemistry of hepatic phosphatases of a physiologic pH; with special reference to the demonstration of bile canaliculi.

Authors: M WACHSTEIN; E MEISEL
Journal: Am J Clin Pathol Date: 1957-01 Impact factor: 2.493

2. Protein measurement with the Folin phenol reagent.

Authors: O H LOWRY; N J ROSEBROUGH; A L FARR; R J RANDALL
Journal: J Biol Chem Date: 1951-11 Impact factor: 5.157

3. Nonenzymatic formation of guanosine 3':5'-monophosphate from guanosine triphosphate.

Authors: H Kimura; F Murad
Journal: J Biol Chem Date: 1974-01-10 Impact factor: 5.157

4. Electron microscopic demonstration of insulin receptors on adipocyte plasma membranes utilizing a ferritin-insulin conjugate.

Authors: L Jarett; R M Smith
Journal: J Biol Chem Date: 1974-11-10 Impact factor: 5.157

5. A highly sensitive adenylate cyclase assay.

Authors: Y Salomon; C Londos; M Rodbell
Journal: Anal Biochem Date: 1974-04 Impact factor: 3.365

6. The glucagon-sensitive adenyl cyclase system in plasma membranes of rat liver. V. An obligatory role of guanylnucleotides in glucagon action.

Authors: M Rodbell; L Birnbaumer; S L Pohl; H M Krans
Journal: J Biol Chem Date: 1971-03-25 Impact factor: 5.157

7. Lead ion and phosphatase histochemistry. I. Nonenzymatic hydrolysis of nucleoside phosphates by lead ion.

Authors: A S Rosenthal; H L Moses; D L Beaver; S S Schuffman
Journal: J Histochem Cytochem Date: 1966-10 Impact factor: 2.479

8. The use of dextran in phosphatase techniques employing lead salts.

Authors: S Szmigielski
Journal: J Histochem Cytochem Date: 1971-08 Impact factor: 2.479

9. Method for the isolation of intact islets of Langerhans from the rat pancreas.

Authors: P E Lacy; M Kostianovsky
Journal: Diabetes Date: 1967-01 Impact factor: 9.461

10. Biochemical characterization and cytochemical localization of a catecholamine-sensitive adenylate cyclase in isolated capillary endothelium.

Authors: R C Wagner; P Kreiner; R J Barrnett; M W Bitensky
Journal: Proc Natl Acad Sci U S A Date: 1972-11 Impact factor: 11.205

33 in total

1. A new dynamic model system for the study of capture reactions for diffusable compounds in cytochemistry. III. Influence of the matrix composition on the lead phosphate precipitation process in acid phosphatase cytochemistry.

Authors: A S De Jong; T J Hak; P Van Duijn; W T Daems
Journal: Histochem J Date: 1979-03

7. Ultracytochemical localizations of adenylate cyclase, guanylate cyclase and cyclic 3',5'-nucleotide phosphodiesterase activity on the trophoblast in the human placenta. Direct histochemical evidence.

Authors: S Matsubara; T Tamada; T Saito
Journal: Histochemistry Date: 1987

8. Electron microscopical demonstration of adenylate cyclase activity in nervous tissue.

Authors: L Rechardt; M Härkönen
Journal: Histochemistry Date: 1977-03-04

9. Adenylate cyclase in the microvessels of the rat brain. A histochemical study with light and electron microscopy.

Authors: G Szumańska; A Palkama; J I Lehtosalo; H Uusitalo
Journal: Acta Neuropathol Date: 1984 Impact factor: 17.088

10. Specificity of cytochemical demonstration of adenylate cyclase in liver using adenylate-(beta, gamma-methylene) diphosphate as substrate.

Authors: D Mayer; V Ehemann; H J Hacker; F Klimek; P Bannasch
Journal: Histochemistry Date: 1985