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High yielding recombinant Staphylokinase in bacterial expression system-cloning, expression, purification and activity studies.

Protein Expr Purif.. 2009-03;  64(1):69-75
Mandi N, Soorapaneni S, Rewanwar S, Kotwal P, Prasad B, Mandal G, Padmanabhan S. Biotechnology R & D, Lupin Limited, 46A/47A, Nande Village, Mulshi Taluka, Lupin Research Park, Pune-411042, India
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摘要

Staphylokinase (SAK) is emerging as an important thrombolytic agent. In this report, we describe the cloning, expression, purification and activity studies of the SAK gene of Staphylococcus aureus from a custom synthesised SAK gene. The SAK gene of 411 bp yielded a protein of ∼15 kDa when expressed under pET21a vector using IPTG as an inducer in BL21 (DE3) pLysE codon Plus cells. The recombinant SAK (rSAK) was soluble in nature and constituted nearly 35% of the total cellular protein as estimated by densitometry scanning. Fermentation studies were carried out to optimize various parameters for maximizing the yield of rSAK and with the optimized medium, the yield of rSAK was nearly 2.8 g/L of ... More

关键词

Staphylococcus aureus; Staphylokinase; Cloning; T7 promoter; Expression; PG activation; Chromogenic substrate assay