LIPOPOLYSACCHARIDE-SENSITIVE SERINE-PROTEASE ZYMOGEN (FACTOR C) OF LIMULUS HEMOCYTES: IDENTIFICATION AND ALIGNMENT OF PROTEOLYTIC FRAGMENTS PRODUCED DURING THE ACTIVATION SHOW THAT IT IS A NOVEL TYPE OF SERINE-PROTEASE

F Tokunaga; T Miyata; T Nakamura; T Morita; S Iwanaga

doi:10.1055/s-0038-1644609

Subscribe to RSS

Please copy the URL and add it into your RSS Feed Reader.

https://www.thieme-connect.de/rss/thieme/en/10.1055-s-00035024.xml

Share / Bookmark

Facebook Linkedin Weibo

Download PDF

Thromb Haemost 1987; 58(01): 490
DOI: 10.1055/s-0038-1644609

Abstracts

COAGULATION: GENERAL

Schattauer GmbH Stuttgart

LIPOPOLYSACCHARIDE-SENSITIVE SERINE-PROTEASE ZYMOGEN (FACTOR C) OF LIMULUS HEMOCYTES: IDENTIFICATION AND ALIGNMENT OF PROTEOLYTIC FRAGMENTS PRODUCED DURING THE ACTIVATION SHOW THAT IT IS A NOVEL TYPE OF SERINE-PROTEASE

F Tokunaga

Department of Biology, Faculty of Science, Kyushu University 33, Fukuoka, Japan

,

T Miyata

Department of Biology, Faculty of Science, Kyushu University 33, Fukuoka, Japan

,

T Nakamura

Department of Biology, Faculty of Science, Kyushu University 33, Fukuoka, Japan

,

T Morita

Department of Biology, Faculty of Science, Kyushu University 33, Fukuoka, Japan

,

S Iwanaga

Department of Biology, Faculty of Science, Kyushu University 33, Fukuoka, Japan

› Author Affiliations

Further Information

Publication History

Publication Date:
23 August 2018 (online)

Also available at

PDF Download Permissions and Reprints

Limulus clotting factor, factor C, is a lipopolysaccharide (LPS)-sensitive serine-protease zymogen present in the hemocytes. It is a two-chain glycoprotein (M.W. = 123,000) composed of a heavy chain (M.W. = 80,000) and a light chain (M.W. = 43,000) T. Nakamura et al. (1986) Eur. J. Biochem. 154, 511-521 .

On further studies of this zymogen, a single-chain factor C (M.W. = 123,000) was identified by Western blotting technique. The heavy chain had an NH₂-terminal sequence of Ser-Gly-Val-Asp-, which was consistent with the NH₂-terminal sequence of the single-chain factor C, indicating that the heavy chain is located in the NH₂-terminal part of the zymogen. The light chain had an NH₂2-terminal sequence of Ser-Ser-Gln-Pro-. Incubation of the two-chain zymogen with LPS resulted in the cleavage of a Phe-Ile bond between residues 72 and 73 of the light chain. Concomitant with this cleavage, the A (72.amino acids) and B chains derived from the light chain was formed. The complete amino acid sequence of the A chain was determined by automated Edman degradation. The A chain contained a typical segment which is similar structuraly to those a family of repeats in human β₂ -glycoprotein I, complement factors B, Clr, Cls, H, C4b-binding protein, 02, coagulation factor XIII b subunit, haptoglobin a chain, and interleukin 2 receptor. The NH₂-terminal sequence of the B chain was Ile-Trp-Asn-Gly-. This chain contained the serine-active site sequence of -ASP-Ala-Cys-Ser-Gly-Asp-SER-Gly-Gly-Pro-.

These results indicate that limulus factor C exists in the hemocytes in a single-chain zymogen form and is converted to an active serine-protease by hydrolysis of a specific Phe-Ile peptide bond. The correlation of limulus factor C and mammalian complement proteins was also suggested.