Activation of calpain in lens: a review and proposed mechanism.

Abstract:

:The purpose of these experiments was to develop a hypothesis to explain activation of m-calpain in cataractogenesis observed in rodents. The in vitro model used to study m-calpain activation was to correlate breakdown of the 'reporter' protein alpha-crystallin with the appearance of activated m-calpain using protein sequencing and casein zymography. Incubation of alpha-crystallins with m-calpain and Ca2+ caused proteolysis of alpha-crystallins and accumulation of new polypeptides. E64 and calpain inhibitor I each inhibited proteolysis of alpha-crystallins. The N-terminus of the 80 kDa subunit of m-calpain was blocked at time 0 (pro calpain). After incubation with Ca2+, the remaining 80 kDa subunit of m-calpain gave a N-terminal sequence of KDREAAEGLG, indicating loss of nine amino acid from the N-terminus (autolysed calpain). The new 43 kDa m-calpain fragment also gave a N-terminal sequence of KDREAAEGLG, indicating the same loss of the first nine amino acids on the N-terminus as well as a major loss of the C-terminal half of the subunit (degraded calpain). In contrast, the N-terminus of the 80 kDa subunit of m-calpain remained blocked when E64 was present (unautolysed form). Moreover, the Ca2+ concentration required for proteolysis decreased when calpain was pre-incubated with Ca2+, although proteolysis of alpha-crystallin required a higher Ca2+ concentration than proteolysis of casein. These data suggested that the sequence of events for m-calpain activation were unautolysed, autolysed and finally degraded calpain. Unautolysed and/or autolysed calpains may be proteolytically active against alpha-crystallin.

journal_name

Exp Eye Res

authors

Azuma M,Fukiage C,David LL,Shearer TR

doi

10.1006/exer.1996.0234

subject

Has Abstract

pub_date

1997-04-01 00:00:00

pages

529-38

issue

4

eissn

0014-4835

issn

1096-0007

pii

S0014-4835(96)90234-1

journal_volume

64

pub_type

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