首页> 美国卫生研究院文献>Biochemical Journal >Enzymic transfer of glucose and xylose from uridine diphosphate glucose and uridine diphosphate xylose to bilirubin by untreated and digitonin-activated preparations from rat liver
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Enzymic transfer of glucose and xylose from uridine diphosphate glucose and uridine diphosphate xylose to bilirubin by untreated and digitonin-activated preparations from rat liver

机译:葡萄糖和木糖的尿素二磷酸葡萄糖和尿苷二磷酸木糖的葡萄糖和酶的未处理和洋地黄素活化的大鼠肝脏制剂的酶促转移

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摘要

1. Digitonin-treated and untreated homogenates, cell extracts and washed microsomal preparations from liver of Wistar R rats are capable of transferring sugar from UDP-glucose or UDP-xylose to bilirubin. No formation of bilirubin glycosides occurred with UDP-galactose or d-glucose, d-xylose or d-glucuronic acid as the sources of sugar. 2. Procedures to assay digitonin-activated and unactivated bilirubin UDP-glucosyltransferase and bilirubin UDP-xylosyltransferase were developed. 3. In digitonin-activated microsomal preparations the transferring enzymes had the following properties. Both enzyme activities were increased 2.5-fold by pretreatment with digitonin. They were optimum at pH6.6–7.2. Michaelis–Menten kinetics were followed with respect to UDP-glucose. In contrast, double-reciprocal plots of enzyme activity against the concentration of UDP-xylose showed two intersecting straight-line sections corresponding to concentration ranges where either bilirubin monoxyloside was formed (at low UDP-xylose concentrations) or where mixtures of both the mono- and di-xyloside were synthesized (at high UDP-xylose concentrations). Both enzyme activities were stimulated by Mg2+; Ca2+ was slightly less, and Mn2+ slightly more, stimulatory than Mg2+. Of the activities found in standard assay systems containing Mg2+, 58–78% (substrate UDP-glucose) and 0–38% (substrate UDP-xylose) were independent of added bivalent metal ion. Double-reciprocal plots of the Mg2+-dependent activities against the concentration of added Mg2+ were linear. 4. In comparative experiments the relative activities of liver homogenates obtained with UDP-glucuronic acid, UDP-glucose and UDP-xylose were 1:1.5:2.7 for untreated preparations and 1:0.29:0.44 after activation with digitonin. 5. Bilirubin UDP-glucuronyltransferase was protected against denaturation by human serum albumin, whereas bilirubin UDP-xylosyltransferase was not. 6. Digitonin-treated and untreated liver homogenates from Gunn rats were inactive in transferring sugar to bilirubin from UDP-glucuronic acid (in agreement with the work of others), UDP-glucose or UDP-xylose.
机译:1.来自维斯塔R大鼠肝脏的洋地黄酮处理过的和未经处理的匀浆,细胞提取物和洗涤过的微粒体制剂能够将糖从UDP-葡萄糖或UDP-木糖转移至胆红素。以UDP-半乳糖或d-葡萄糖,d-木糖或d-葡萄糖醛酸作为糖源,未发生胆红素糖苷的形成。 2.制定了测定洋地黄素激活和未激活的胆红素UDP-葡萄糖基转移酶和胆红素UDP-木糖基转移酶的程序。 3.在洋地黄酮活化的微粒体制剂中,转移酶具有以下特性。用洋地黄皂苷预处理可使两种酶的活性提高2.5倍。它们在pH6.6–7.2最佳。对于UDP-葡萄糖,遵循了Michaelis-Menten动力学。相比之下,酶活性相对于UDP-木糖浓度的双倒数图显示了两个相交的直线部分,对应于浓度范围,在该浓度范围内形成了胆红素单氧体苷(在低UDP-木糖浓度下)或两种单-合成了二木糖苷和二木糖苷(在高UDP-木糖浓度下)。 Mg 2 + 刺激了两种酶的活性。 Ca 2 + 比Mg 2 + 少,而Mn 2 + 少。在包含Mg 2 + 的标准测定系统中发现的活性中,58-78%(底物UDP-葡萄糖)和0-38%(底物UDP-木糖)与添加的二价金属离子无关。 Mg 2 + 依赖性活性与添加的Mg 2 + 浓度的双倒数图呈线性关系。 4.在对比实验中,未经处理的制剂用UDP-葡萄糖醛酸,UDP-葡萄糖和UDP-木糖得到的肝匀浆的相对活性为1:1.5:2.7,而用洋地黄皂苷激活后的肝匀浆的相对活性为1:0.29:0.44。 5.胆红素UDP-葡萄糖醛酸转移酶可防止人血清白蛋白变性,而胆红素UDP-木糖基转移酶则不能。 6.来自Gunn大鼠的洋地黄素处理过的和未经处理的肝匀浆均无活性,无法将糖从UDP-葡萄糖醛酸(与他人的工作),UDP-葡萄糖或UDP-木糖转移至胆红素中。

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