Structure and function of microplasminogen: I. Methionine shuffling, chemical proteolysis, and proenzyme activation

Abstract

We have cloned and expressed microplasminogen (mPlg), consisting of the N-terminal undecapeptide of human glu-P/g spliced to its proenzyme domain. This truncated (∼28 kDa) proenzyme retained the distinctive catalytic activities of the larger parent. Replacement of M residues followed by M shuffling permitted subsequent scission by site-directed chemical proteolysis (in CNBr/formic acid) without impairing any of the protein's characteristic properties. Activation of chymotrypsinogen-related zymogens occurs by limited proteolysis; the newly liberated, highly conserved N-terminus (VVGG) forms a salt bridge with an aspartyl residue immediately upstream of the active site serine. The role of both of these elements in mPlg activation was probed using protein engineering and site-directed proteolysis to alter the length and amino acid composition of the N-terminus, and to replace the aspartate. All modifications affected both K_m and k_cat The results identify some structural parameters of the N-terminus required for proenzyme activation.