شماره ركورد
478516
عنوان مقاله
بهينه سازي بيان ژن و تخليص پروتئين نوتركيب LTB باكتري اشريشيا كلي انتروتوكسيژنيك و توليد آنتي بادي عليه آن
عنوان به زبان ديگر
Optimization of gene expression and purification of enterotoxigenic Escherichia coli recombinant LTB protein and antibody production against it
پديد آورندگان
اماني، جعفر نويسنده amani, jafar , منصوري، ميثم نويسنده دانشگاه امام حسين تهران,دانشكده علوم پايه mansouri, meysam , احصايي، زهرا نويسنده دانشگاه امام حسين تهران,دانشكده علوم پايه Ehsaei , zahra , موذني ، محمد نويسنده moazeni, mohammad , سليميان، جعفر نويسنده دانشگاه امام حسين (ع),دانشكده علوم پايه , , نظريان، شهرام نويسنده Nazarian , shahram , خالصي، راضيه نويسنده دانشگاه امام حسين تهران,دانشكده علوم پايه ,
رتبه نشريه
-
تعداد صفحه
7
از صفحه
141
تا صفحه
147
كليدواژه
زيرواحد B توكسين حساس به حرارت , آنتي بادي , بهينه سازي بيان ژن , اشريشيا كلي انتروتوكسيژنيك , واكسن نوتركيب
چكيده لاتين
Aims: It has been estimated that gastroenteritis is caused by bacteria in 30-70% of cases. Enterotoxigenic Escherichia coli or ETEC is one of the most common agents causing diarrhea. Protective immunity may be induced against this disease. Designing and producing a vaccine against this disease is one of the purposes of World Health Organization. Vaccine candidate molecules have to induce protective immunity against a broad spectrum of ETEC bacteria. Most ETEC strains can produce labile toxin; therefore labile toxin may be a proper candidate for being used as a vaccine molecule. The aim of this study was to optimize Heat-labile Toxin B Subunit expression in order to investigate its immunological properties.
Materials & Methods: Optimizing of 3 parameters (IPTG concentration, time and temperature of promoter induction) was performed. Recombinant protein was purified with Ni-NTA column. Purified Heat-labile Toxin B Subunit was injected to mice subcutaneously in 4 sessions. Blood samples were taken during the interval between the injections and after last injection. Then, ELISA was performed.
Results: The optimum expression occurred at ImM IPTG concentration, after 3 hours and at 37°C. Recombinant protein was highly purified (>95%) with Ni-NTA column. Also, ELISA showed high titer of antibody production in mice.
Conclusion: Expressed Heat-labile Toxin B Subunit is an immunogenic protein and can be one of the important components in vaccine development against ETEC.
Keywords: Enterotoxigenic Escherichia coli, Heat-Labile Toxin B Subunit, Expression, Recombinant Vaccine, Antibody
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