Molecular cloning and expression of S1 glycoprotein gene of infectious bronchitis virus (IBV) isolate IRFIBV32 in Lactococcus lactis

سال انتشار: 1397
نوع سند: مقاله کنفرانسی
زبان: انگلیسی
مشاهده: 315

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شناسه ملی سند علمی:

CMTS02_029

تاریخ نمایه سازی: 29 تیر 1398

چکیده مقاله:

Avian infectious bronchitis virus (IBV) is a highly infectious pathogen in chickens causing acute, highly contagious respiratory disease [1]. S1 glycoprotein protein, a majorstructural protein of IBV, is responsible for IBV pathogenesis [2]. Lactococcus lactis bacteria can be used to create mucosal recombinant vaccines [3]. In this study, the S1 glycoprotein gene of infectious bronchitis virus isolate IRFIBV32 was amplified by RT-PCR using two pairs of primers and ligated to pTZ57R/T and pTG-19T vectors. Then, the resulting plasmids (pTZ57-S1 and pTG-19-S1) were transformed to competent E.coli GM2163. pNZ8110 and pNZ8148 L. lactis expression vectors for secretory and cytoplasmic heterologous protein were selected. Then, S1 gene fragment cloned into these vectors and pNZ8110-S1/S and pNZ8148-S1/C plasmids were yield for secretory and cytoplasmic protein production, respectively, in E. coli MC1061. After preliminary transformation into E. coli MC1061, the plasmids were extracted and transformed to L. lactis NZ9000 by electroporation. During each step the location and accuracy of genes sequence were confirmed by PCR, restriction enzyme analysis and sequencing. SDS-PAGE of purified intra and extracellular expression of S1 protein from recombinant bacteria revealed that the S1 was successfully expressed in cytoplasmic and secretory forms.

نویسندگان

Seyedeh Alemeh Hosseinian

Department of Clinical Sciences, School of Veterinary Medicine, Shiraz University, Shiraz, Iran

Arsalan Hosseini

Department of Pathobiology, School of Veterinary Medicine, Shiraz University, Shiraz, Iran

Keramat Asasi

Department of Clinical Sciences, School of Veterinary Medicine, Shiraz University, Shiraz, Iran