Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI

A molecular cloning of African swine fever virus k205r and b602l genes in £ coli was carried out. The expression and purification conditions ensuring high yield of recombinant proteins were optimized. Dissolved recombinant proteins were purified by metal-chelate affinity chromatography using Ni-NTA-...

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Main Authors: A. V. Scherbakov, A. S. Yakovleva, A. M. Timina, M. R. Yakupov
Format: Article
Language:English
Published: Da Vinci Media 2018-04-01
Series:Ветеринария сегодня
Subjects:
Online Access:https://veterinary.arriah.ru/jour/article/view/191
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author A. V. Scherbakov
A. S. Yakovleva
A. M. Timina
M. R. Yakupov
author_facet A. V. Scherbakov
A. S. Yakovleva
A. M. Timina
M. R. Yakupov
author_sort A. V. Scherbakov
collection DOAJ
description A molecular cloning of African swine fever virus k205r and b602l genes in £ coli was carried out. The expression and purification conditions ensuring high yield of recombinant proteins were optimized. Dissolved recombinant proteins were purified by metal-chelate affinity chromatography using Ni-NTA-agarose («Qiagen»). Recombinant antigens are biologically safe, easier to prepare and ensure higher ELISA specificity. The purified protein yield from 100 ml off. coli culture was 1,5 mg for pK205R and 2 mg for pB602L.
format Article
id doaj-art-01a098b701494b52905585290ba7c90d
institution Kabale University
issn 2304-196X
2658-6959
language English
publishDate 2018-04-01
publisher Da Vinci Media
record_format Article
series Ветеринария сегодня
spelling doaj-art-01a098b701494b52905585290ba7c90d2025-02-06T09:52:05ZengDa Vinci MediaВетеринария сегодня2304-196X2658-69592018-04-01023135191Cloning and expression of African swine fever virus K205R and B602L genes inf. COLIA. V. Scherbakov0A. S. Yakovleva1A. M. Timina2M. R. Yakupov3FGBI "ARRIAH", VladimirFGBI "ARRIAH", VladimirFGBI "ARRIAH", VladimirFGBI "ARRIAH", VladimirA molecular cloning of African swine fever virus k205r and b602l genes in £ coli was carried out. The expression and purification conditions ensuring high yield of recombinant proteins were optimized. Dissolved recombinant proteins were purified by metal-chelate affinity chromatography using Ni-NTA-agarose («Qiagen»). Recombinant antigens are biologically safe, easier to prepare and ensure higher ELISA specificity. The purified protein yield from 100 ml off. coli culture was 1,5 mg for pK205R and 2 mg for pB602L.https://veterinary.arriah.ru/jour/article/view/191african swine fever viruspk205r and pb602l recombinant proteinsexpression
spellingShingle A. V. Scherbakov
A. S. Yakovleva
A. M. Timina
M. R. Yakupov
Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
Ветеринария сегодня
african swine fever virus
pk205r and pb602l recombinant proteins
expression
title Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
title_full Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
title_fullStr Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
title_full_unstemmed Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
title_short Cloning and expression of African swine fever virus K205R and B602L genes inf. COLI
title_sort cloning and expression of african swine fever virus k205r and b602l genes inf coli
topic african swine fever virus
pk205r and pb602l recombinant proteins
expression
url https://veterinary.arriah.ru/jour/article/view/191
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