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GloboZymes/c-Jun, Proto-Oncogene/10μg/GLO127-010

价格
¥13300.00
货号:GLO127-010
浏览量:127
品牌:GloboZymes
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商品描述

c-Jun, Proto-Oncogene

Source: Recombinant human produced in E. coli

Purity: > 90% by SDS-PAGE, apparent Mr ~ 39-kDa

Supplied: In 50 μl of 50 mM Tris-HCl pH 7.0 buffer containing 14 mM β-mercaptoethanol, 1 mM benzamidine, 0.1 mM phenylmethanesulfonyl fluoride, 1 mM EDTA and 10% glycerol. Maintain in aliquots at -70° C. Avoid repeated thawing.

GloboZymes c-Jun preparations are suitable for studies on the kinetics, enzymology, functional significance and regulation of the phosphorylation of this important proto-oncogene. The purified preparations are effective as substrate for JNK/SAPK, MAPK, GSK-3 and CK-2 among other protein kinases.

Background: The proto-oncogene c-Jun is an important transactivating factor. It is a component of the AP-1 and ATF-2 transcription factors. A wide variety of cellular signals regulate c-Jun acutely via modulation of its phosphorylation state. Phosphorylation can both inhibit and activate the proto-oncogene. GSK-3 phosphorylates c-Jun at a region proximal to the highly basic DNA binding domain (Thr239/Ser243/Ser249). This phosphorylation prevents DNA association with c-Jun homodimers, but not with c-Jun-c-Fos heterodimers. In contrast, phosphorylation by JNK/SAPK at Ser63 and Ser73, in a region proximal to the transactivation domain, activates the c-Jun/AP-1 and c-Jun/ATF2 transcriptional activator complexes to induce a number of genes. The MAP kinases ERK1 and ERK2  phosphorylate c-Jun at Thr91/Thr93/Thr95. However, the significance of these phosphorylations is uncertain.

Figure: A purified preparation of recombinant human c-Jun was subjected to SDS-PAGE. The gel was stained with Coomassie Blue.

References: Al-Murrani SW et al (1999)  Biochem J 341, 293-298; Karin M (1995)  J Biol Chem 270, 16483-16486; Woodgett JR et al (1996) Phil Trans R Soc Lond 351, 135-141; Kyriakis JM & Avruch J (2001)  Physiol Rev 81, 807-869

GloboZymes的eIF4E(S53A)来源:在大肠杆菌中产生的重组人 纯度:通过SDS-PAGE大于90%,表观先生〜28-kDa提供:在50μl的50 mM Tris-HCl pH 7.0缓冲液中,其中含有14 mMβ-巯基乙醇,1 mM苯甲am,0.1 mM苯基甲磺酰氟,1 mM EDTA和10%甘油。等分试样保持在-70°C下。避免重复解冻。别名:丙氨酸突变体的真核蛋白合成起始因子4E丝氨酸53;eIF-4E S53A。eIF4ES53A背景:mRNA Cap结合蛋白合成起始因子4E(eIF4E)参与了蛋白合成的早期限速步骤。eIF4E的过表达导致细胞转化和肿瘤发生,并发生在许多癌细胞中。在静止细胞中,eIF4E作为与4EBP结合蛋白的非活性复合物存在。响应胰岛素和其他细胞外刺激,eIF4E与4EBP分离并被募集到活性eIF4F复合体中。活性eIF4F复合体除eIF4E外还包含eIF4A和eIF4G。响应胰岛素和其他生长因子,eIF4E在Ser209处被磷酸化。这种磷酸化增强了eIF4E对加帽的mRNA的亲和力。它是由丝裂素激活的蛋白激酶(MAPK)相互作用激酶(Mnk's)催化的。它也被称为cPK的胰岛素刺激的激酶催化,该激酶也使Thr210在起始因子上磷酸化。 图:纯化的eIF4E(S53A)制剂的SDS-PAGE模式。凝胶用考马斯蓝染色。