The recruitment of blood coagulation factor X into snake venom gland as a toxin - The role of promoter Cis-elements in its expression

Journal:Thrombosis and Haemostasis
ISSN:0340-6245
DOI:http://dx.doi.org/10.1160/TH09-03-0162
Issue:2009: 102/3 (Sep) pp. 421-610
Pages:469-478

The recruitment of blood coagulation factor X into snake venom gland as a toxin - The role of promoter Cis-elements in its expression

Shiyang Kwong1; Anthony E. Woods2; Peter J. Mirtschin2,3; Ruowen Ge1; R. Manjunatha Kini1,4

1Department of Biological Sciences, Faculty of Science, National University of Singapore, Singapore, Singapore; 2Sansom Institute, School of Pharmacy and Medical Sciences, University of South Australia, Adelaide, South Australia, Australia; 3Venom Supplies Pty Ltd, Tanunda, South Australia, Australia; 4Department of Biochemistry, VCU Medical Center, Virginia Commonwealth University, Richmond, Virginia, USA

Summary

Trocarin D is a prothrombin activator from the Tropidechis carinatus venom. It is a functional and structural homologue to mammalian blood coagulation factor Xa. Trocarin D is hypothesised to have evolved from its factor X counterpart (TrFX) through gene duplication and recruitment. The genes of trocarin D and TrFX have significant sequence identities, except for insertions/ deletions in their intron 1 and promoter regions. In trocarin D intron 1 region, there are three insertions and two deletions. In trocarin D promoter region, there is a novel 264 bp insertion which has potential cis-elements. This insertion is termed as Venom Recruitment/Switch Element (VERSE) and is hypothesised to account for switching the low-level constitutive expression of factor X in the liver to the high-level inducible expression of trocarin D in the venom gland. To understand the role of VERSE in the trocarin D expression, its cis-elements were characterised by luciferase assays in mammalian cell lines as well as snake venom gland cells. The ability of VERSE to drive luciferase expression is comparable to that of the trocarin D promoter. The predicted cis-elements are important in promoting expression as their mutagenesis resulted in lower luciferase expression. VERSE minimal core promoter and three novel cis-elements (two up-regulatory and one suppressor elements) were identified using deletion/site-directed mutagenesis studies. VERSE is primarily responsible for the increase of trocarin D expression. The insertions/deletions within trocarin D intron 1 need to be characterised for their role in tissue-specific and inducible expression of trocarin D.

Keywords

factor X, promoter, prothrombin activator, recruitment, snake venom

DOI

http://dx.doi.org/10.1160/TH09-03-0162

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