AI Article Synopsis

  • Calpains are important intracellular enzymes that regulate multiple cellular functions, and their improper activation can lead to serious health issues like muscular dystrophies and tumors.
  • nCL-2/calpain 8 is mainly found in the stomach and is involved in membrane trafficking of gastric surface mucus cells, but its specific enzymatic properties haven’t been thoroughly studied.
  • In this research, nCL-2 was successfully produced and purified, showing Ca(2+)-dependent activity and distinct forms of oligomerization, indicating a unique regulatory mechanism different from other calpains.

Article Abstract

Calpains constitute a family of intracellular Ca(2+)-regulated cysteine proteases that are indispensable in the regulation of a wide variety of cellular functions. The improper activation of calpain causes lethality or various disorders, such as muscular dystrophies and tumor formation. nCL-2/calpain 8 is predominantly expressed in the stomach, where it appears to be involved in membrane trafficking in the gastric surface mucus cells (pit cells). Although the primary structure of nCL-2 is quite similar to that of the ubiquitous m-calpain large subunit, the enzymatic properties of nCL-2 have never been reported. Here, to characterize nCL-2, the recombinant protein was prepared using an Escherichia coli expression system and purified to homogeneity. nCL-2 was stably produced as a soluble and active enzyme without the conventional calpain regulatory subunit (30K). Purified nCL-2 showed Ca(2+)-dependent activity, with half-maximal activity at about 0.3 mM Ca(2+), similar to that of m-calpain, whereas its optimal pH and temperature were comparatively low. Immunoprecipitation analysis revealed that nCL-2 exists in both monomeric and homo-oligomeric forms, but not as a heterodimer with 30K or 30K-2, and that the oligomerization occurs through domains other than the 5EF-hand domain IV, most probably through domain III, suggesting a novel regulatory system for nCL-2.

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Source
http://dx.doi.org/10.1074/jbc.M703168200DOI Listing

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