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人白介素18受体(IL-18R)elisa试剂盒

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  • 公司名称厦门仑昌硕生物科技有限公司
  • 品       牌其他品牌
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  • 所  在  地厦门市
  • 厂商性质生产厂家
  • 更新时间2020/4/26 16:42:45
  • 访问次数660
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厦门仑昌硕生物科技有限公司集研发、生产、销售、服务及品牌代理为一体的生物技术公司,目前可提供各种抗体、免疫学相关的检测试剂盒、胎牛血清,动物抗血清等高品质产品及服务,涵盖分子生物学、细胞生物学、免疫学等生命科学领域。
公司非常注重企业信息化的建设及企业平台的建设,我们内部采用了*的信息处理平台,保证客户的需求可以准确、高效处理。
公司成立之初,立足外贸,和部分欧美及亚非国家的客户建立了良好的合作,随着国内生物领域的蓬勃发展,逐步把重心转移到国内来,为每一位科研人员献上高品质的产品及服务是我们的使命。

集研发、生产、销售、服务及品牌代理为一体的生物技术公司,目前可提供各种抗体、免疫学相关的检测试剂盒、胎牛血清,动物抗血清等高品质产品及服务,涵盖分子生物学、细胞生物学、免疫学等生命科学领域。
产地 国产 级别 其他
Porcine IL-12Rβ2 gene was cloned from mRNA preparation of mitogen-activated peripheral blood mononuclear cells (PBMCs), and its complete nucleotide sequence was determined. To confirm the biological f
人白介素18受体(IL-18R)elisa试剂盒 产品信息

Porcine IL-12Rβ2 gene was cloned from mRNA preparation of mitogen-activated peripheral blood mononuclear cells (PBMCs), and its complete nucleotide sequence was determined. To confirm the biological function, the entire open reading frame (ORF) was re-cloned into a mammalian expression vector, pcDNA3.1/Zeo(+), at the downstream of CMV promoter, and introduced to a Th1-like human lymphoma cell line, Jurkat E6-1. Antibiotic-resistant cells retaining the expression construct were selected then, isolated by the limiting dilution method. An established clone (10B10) constitutively expressed chimeric IL-12Rs composed of intrinsic (human) β1 and extrinsic (porcine) β2 subunits, and produced interferon (IFN)-γ in response to IL-12 of both species with optimal PHA/PMA stimulation. The production of IFN-γ was observed as early as 42 h after culture and appeared to be dose-dependent within the range between 20 and 2000 pg/ml. Thus, this clone not only reacts with IL-12 of both species but also provides a useful tool for quick and sensitive detection of IL-12 bioactivity.Porcine IL-12Rβ2 gene was cloned from mRNA preparation of mitogen-activated peripheral blood mononuclear cells (PBMCs), and its complete nucleotide sequence was determined. To confirm the biological function, the entire open reading frame (ORF) was re-cloned into a mammalian expression vector, pcDNA3.1/Zeo(+), at the downstream of CMV promoter, and introduced to a Th1-like human lymphoma cell line, Jurkat E6-1. Antibiotic-resistant cells retaining the expression construct were selected then, isolated by the limiting dilution method. An established clone (10B10) constitutively expressed chimeric IL-12Rs composed of intrinsic (human) β1 and extrinsic (porcine) β2 subunits, and produced interferon (IFN)-γ in response to IL-12 of both species with optimal PHA/PMA stimulation. The production of IFN-γ was observed as early as 42 h after culture and appeared to be dose-dependent within the range between 20 and 2000 pg/ml. Thus, this clone not only reacts with IL-12 of both species but also provides a useful tool for quick and sensitive detection of IL-12 bioactivity.

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