THE STUDY OF (△N)A21 INSULIN

WANG Chun-yang 1,WANG Qiu-fang 2 (1.College of Animal Science and Technology,Shangdong Agricutural University, Taian, 271018; 2.College of Animal Science and Animal Medicine,Northwest Agricutural University, Yangling,712100 )

N)A21proinsulin;dispartion and purification;cleavage; Radioimmuno assay(RIA);receptobing assay(RBA)

In this paper, (△N)A21Proinsulin was directly inserted into the multiple cloning site-EcoRI and BamHI, and the resulting plasmid was used to transform E.coil strain DH 5α (△N) A21Proinsulin have been expressed and the expressing rate is 8%～15%. The target proinsulin was obtained with highly purity by series of processing, which consists of disintegration cell membrane,the fission of inclusion body and other steps. After cheavaged by trypsin and carboxypeptidase B, (△N) A21Proinsulin was transformed into corresponding mutant insulin. (△N) A21insulin was analyzed by Native-PAGE, Radioimmuno Assay (RIA), recptor binging assay (RBA). According to the result, the activity of (△N) A21proinsulin is muchlower than natural insulin. This result implies that A21 is very important for insulin to sustain certain spatial conformation. A21Asn isn't an important amino acid which is bound with insulin receptor, but the absention of A21Asn will the affect total activity of insulin. Therefore, A21Asn can be replaced by other amino acids but it can't be absent.