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Characterization of the zinc-metalloprotein nature of rat spermatidal protein TP2

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dc.contributor.author Kundu, Tapas K
dc.contributor.author Rao, M R S
dc.date.accessioned 2012-02-24T06:50:38Z
dc.date.available 2012-02-24T06:50:38Z
dc.date.issued 1994-08-29
dc.identifier 0014-5793 en_US
dc.identifier.citation FEBS Letters 351(1), 6-10 (1994) en_US
dc.identifier.uri https://libjncir.jncasr.ac.in/xmlui/10572/507
dc.description Restricted Access en_US
dc.description.abstract Spermatidal transition protein, TP2, was purified from rat testes by Hg-affinity chromatography. The present study reports the details of the zinc-metalloprotein nature of TP2 by employing the Zn-65-blotting technique. Chemical modification of cysteine by iodoacetic acid, and histidine by diethylpyrocarbonate, resulted in a near complete inhibition of Zn-65-binding to TP2. The (65)Zinc-binding was localized to the V8 protease-derived N-terminal two-third polypeptide fragment. Circular dichroism spectroscopy studies of TP2 (zinc pre-incubated) and its V8 protease-derived polypeptide fragments revealed that the N-terminal fragment has a Type I-beta-turn spectrum, while the C-terminal fragment has a small but significant alpha-helical structure. EDTA altered the circular dichroism spectrum of TP2 and the N-terminal fragment (zinc binding domain) but not that of the C-terminal fragment. en_US
dc.description.uri http://dx.doi.org/10.1016/0014-5793(94)00799-3 en_US
dc.language.iso en en_US
dc.publisher Elsevier Science BV en_US
dc.rights © 1994 Federation of European Biochemical Societies en_US
dc.subject Spermatidal Transition Protein Tp2 en_US
dc.subject (65)Zinc Blotting en_US
dc.subject Secondary Structure en_US
dc.subject Secondary-Structure en_US
dc.subject Sperm en_US
dc.subject Sequence en_US
dc.title Characterization of the zinc-metalloprotein nature of rat spermatidal protein TP2 en_US
dc.type Article en_US


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