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- 文献和实验
- 技术资料
- 保存条件:
常温,避光
- 克隆性:
单克隆
- 抗体名:
HPGD / PGDH1抗体
抗体类型: Mouse Monoclonal Antibody ( Mouse mAb Service Platform )
克隆号 :
4E2C12E9
抗体宿主 : Mouse IgG1
缓冲液 : 0.2 μm filtered solution in PBS, 5% trehalose may be added in some batches. Please read the hardcopy of COA or contact our customer service to confirm the formulation.
制备方法 : This antibody was produced from a hybridoma resulting from the fusion of a mouse myeloma with B cells obtained from a mouse immunized with purified, E.coli-derived, recombinant human HPGD ( rh HPGD ; Catalog#11205-H08E ; NP_000851.2 ; Met 1 - Gln 266 ). The IgG fraction of the cell culture supernatant was purified by Protein A affinity chromatography.
HPGD / PGDH1抗体背景综述
15-hydroxyprostaglandin dehydrogenase [NAD+], also known as Prostaglandin dehydrogenase 1, HPGD, and PGDH1, is a member of the short-chain dehydrogenases / reductases (SDR) family. Prostaglandins (PGs) play a key role in the onset of labor in many species and regulate uterine contractility and cervical dilatation. Therefore, the regulation of prostaglandin output by PG synthesizing and metabolizing enzymes in the human myometrium may determine uterine activity patterns in human labor both at preterm and at term. Prostaglandin dehydrogenase (PGDH) metabolizes prostaglandins (PGs) to render them inactive. HPGD is down-regulated by cortisol, dexamethasone and betamethasone and down-regulated in colon cancer. It is up-regulated by TGFB1. HPGD contributes to the regulation of events that are under the control of prostaglandin levels. HPGD catalyzes the NAD-dependent dehydrogenation of lipoxin A4 to form 15-oxo-lipoxin A4. and inhibits in vivo proliferation of colon cancer cells. Defects in HPGD are the cause of primary hypertrophic osteoathropathy autosomal recessive (PHOAR) , cranioosteoarthropathy (COA), and isolated congenital nail clubbing.
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xy-0336xy-xyE Monkey IgM/PE荧光素PE标记猴IgM
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xy-0369xy-xyE Rabbit IgM/PE荧光素PE标记兔IgM
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xy-0293xy-Axyxy Rat IgG/APC荧光素APC标记大鼠IgG(细胞流式同型对照)
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文献和实验乙型肝炎、和HBsAg阳性的患者血清中前S1蛋白,前S1抗原阴转愈早,AHB患者的疗程愈短,预后也愈好。说明前S1抗原及其抗体的检测是急性乙型肝炎的临床诊断,疗效观察和判数据预后的良好指标。 前S1蛋白的分子生物学特性 1.乙肝病毒(HBV)的基因结构 HBV为嗜肝DNA病毒,由一个不完全双链DNA组成,约3200个氨基酸。长链L含4个开放读码框架,为病毒蛋白的编码区:S区、C区、P区、X区。短链S相当于长链的50%-100%,其不固定端可被内原性DNA多聚酶延长,使病毒成为完整
纤维素薄膜)上,固相载体以非共价键形式吸附蛋白质,且能保持电泳分离的多肽类型及其生物学活性不变。以固相载体上的蛋白质或多肽作为抗原,与对应的抗 体起免疫反应,再与酶或同位素标记的第二抗体起反应,经过底物显色或放射自显影以检测电泳分离的特异性目的基因表达的蛋白成分。该技术也广泛应用于检测蛋 白水平的表达。二、分类western显色的方法主要有以下几种:i. 放射自显影ii. 底物化学发光ECLiii. 底物荧光ECFiv. 底物DAB呈色现 常用的有底物化学发光ECL和底物DAB呈色,体同水平和实验
,“显色”用标记的二抗。经过PAGE分离的蛋白质样品,转移到固相载体(例如硝酸纤维素薄膜)上,固相载体以非共价键形式吸附蛋白质,且能保持电泳分离的多肽类型及其生物学活性不变。以固相载体上的蛋白质或多肽作为抗原,与对应的抗体起免疫反应,再与酶或同位素标记的第二抗体起反应,经过底物显色或放射自显影以检测电泳分离的特异性目的基因表达的蛋白成分。该技术也广泛应用于检测蛋白水平的表达。二、分类现常用的有底物化学发光ECL和底物DAB呈色,体同水平和实验条件的是用第一种方法,目前发表文章通常是用底物化学发光ECL
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