SIGMA C2139-100MG 胶原酶 来源于溶组织梭菌 9001-12-1
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SIGMA C2139-100MG 胶原酶 来源于溶组织梭菌

9001-12-1
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  • ¥1056
  • Sigma-Aldrich
  • 进口
  • C2139-1G
  • 2025年07月11日
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    • 详细信息
    • 询价记录
    • 文献和实验
    • 技术资料
    • 保存条件

      −20°C

    • 保质期

      根据瓶身LOT号查询

    • 英文名

      Collagenase from Clostridium histolyticum

    • 库存

      有现货

    • 供应商

      浙江羽翔生物科技有限公司

    • CAS号

      9001-12-1

    • 规格

      100MG

    属性

    生物来源

    Clostridium histolyticum

    质量水平

    200

    类型

    Type VIII

    形式

    powder

    比活

    ≥125 CDU/mg solid
    0.5-5.0 FALGPA units/mg solid

    分子量

    68-125 kDa

    适用性

    suitable for release of rat epididymal adipocytes and hepatocytes (for methodology see Type II and Type IV)

    应用

    diagnostic assay manufacturing

    储存温度

    −20°C

    一般描述

    溶组织梭状芽胞杆菌 是一种致病梭状芽胞杆菌,可产生粗胶原酶。这是一种含有胶原酶的混合酶,为非特异性蛋白酶和梭菌蛋白酶。

    应用

    胶原酶可用于:
    • 用于制备动脉组织研究晚期糖基化终产物(AGE),与其他蛋白酶一起用于分解人类肿瘤、小鼠肾脏、人脑、肺上皮细胞等多种组织。在肝脏和肾脏的灌注研究中,胰腺的消化和非实质肝细胞的分离。用于从大鼠肝脏中制备活肝细胞和从大鼠脂肪组织中分离脂肪细胞

    生化/生理作用

    胶原酶由每mol,4g原子钙酶激活。它被乙二醇双(2-氨基乙基醚)四乙酸、β-巯基乙醇、谷胱甘肽、巯基乙suan和8-羟基喹lin所抑制。胶原酶和中性蛋白酶在组织细胞的有效释放中起着重要作用。胶原酶识别序列-R-Pro-8-X-Gly-Pro-R-,其中X表示中性氨基酸。 
    每摩尔胶原蛋白酶被4g原子钙活化。 它被乙二醇-双(β-氨基乙基醚)-N,NN′,N′-四乙酸,β-巯基乙醇、谷胱甘肽、巯基乙suan和8-羟基喹lin抑制。

    单位定义

    一个胶原蛋白消化单元(CDU)从牛跟腱胶原蛋白中释放的肽链量和1.0 μ亮氨酸,5小时,pH7.4,37℃,在钙离子存在下的茚三酮颜色相同。一个 FALGPA水解单元每分钟,25℃,水解1.0 μmole 呋喃基丙烯酰-Leu-Gly-Pro-Ala。一个中性蛋白酶单元水解酪蛋白,产生颜色和1.0 μmole 酪氨酸每5小时,pH7.5,37℃下产生的相同。一个梭菌蛋白酶单元在DTT存在下,pH7.6,25℃,每分钟水解1.0 μmole BAEE。

    分析说明

    也具有梭菌蛋白酶、非特异性中性蛋白酶和胰蛋白酶活性。

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    • 作者
    • 内容
    • 询问日期
    图标文献和实验
    该产品被引用文献

    Liver Immune Cells Release Type 1 Interferon Due to DNA Sensing and Amplify Liver Injury from Acetaminophen Overdose.

    Cells (2018-08-01)
    Alan Moreira de Araujo, Maísa Mota Antunes, Matheus Silvério Mattos, Ariane Barros Diniz, Débora Moreira Alvarenga, Brenda Naemi Nakagaki, Érika de Carvalho, Viviane Aparecida Souza Lacerda, Raquel Carvalho-Gontijo, Jorge Goulart, Kassiana Mafra, Maria Alice Freitas-Lopes, Hortência Maciel de Castro Oliveira, Camila Miranda Dutra, Bruna Araújo David, Aristóbolo Mendes Silva, Valerie Quesniaux, Bernhard Ryffel, Sergio Costa Oliveira, Glen N Barber, Daniel Santos Mansur, Thiago Mattar Cunha, Rafael Machado Rezende, André Gustavo Oliveira, Gustavo Batista Menezes
    PMID30060463
    摘要

    Hepatocytes may rupture after a drug overdose, and their intracellular contents act as damage-associated molecular patterns (DAMPs) that lead to additional leukocyte infiltration, amplifying the original injury. Necrosis-derived DNA can be recognized as a DAMP, activating liver non-parenchymal cells (NPCs). We hypothesized that NPCs react to DNA by releasing interferon (IFN)-1, which amplifies acetaminophen (APAP)-triggered liver necrosis. We orally overdosed different knockout mouse strains to investigate the pathways involved in DNA-mediated amplification of APAP-induced necrosis. Mice were imaged under intravital confocal microscopy to estimate injury progression, and hepatocytes and liver NPCs were differentially isolated for gene expression assays. Flow cytometry (FACS) using a fluorescent reporter mouse estimated the interferon-beta production by liver leukocytes under different injury conditions. We also treated mice with DNase to investigate the role of necrosis DNA signaling in IFN-1 production. Hepatocytes released a large amount of DNA after APAP overdose, which was not primarily sensed by these cells. However, liver NPCs promptly sensed such environmental disturbances and activated several DNA sensing pathways. Liver NPCs synthesized and released IFN-1, which was associated with concomitant hepatocyte necrosis. Ablation of IFN-1 recognition in interferon α/β receptor (IFNAR-/-) mice delayed APAP-mediated liver necrosis and dampened IFN-1 sensing pathways. We demonstrated a novel loop involving DNA recognition by hepatic NPCs and additional IFN-1 mediated hepatocyte death.

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    SIGMA C2139-100MG 胶原酶 来源于溶组织梭菌 9001-12-1
    ¥1056