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GloboZymes/PP2A2, Protein Phosphatase 2A2/5μg/GLO131-005

价格
¥15560.00
货号:GLO131-005
浏览量:127
品牌:GloboZymes
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商品描述

PP2A2, Protein Phosphatase 2A2

Source: Bovine kidney

Purity: > 90% by SDS-PAGE, subunit apparent Mr’s ~ 36- and 65- kDa

Supplied: In 50 μl 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 50% glycerol.

Activity: ~ 2000 units/mg with myelin basic protein (MBP) as substrate. One unit is the amount of PP2A2 that releases 1 nmol of inorganic phosphate from 32P-labeled MBP per min. Maintain preparations in aliquots at -70° C. Avoid repeated thawing.

Synonyms: Protein Phosphatase 2A2; PP2A2

SDS-PAGE of Purified Bovine Kidney PP2A2; Protein Phosphatase 2A2 Background: Protein phosphatase 2A (PP2A) is a divalent cation-independent multifunctional protein serine threonine phosphatase. PP2A regulates numerous cellular processes including the cell cycle, growth and differentiation. Physiological targets of PP2A include cell surface receptors and ion channels, and protein kinases involved in mitogenic signaling and the cell cycle. PP2A also acts on numerous transcription factors as well as key regulatory enzymes in metabolism. PP2A is a growth and tumor suppressor. It is inhibited potently by tumor promoters such as okadaic acid. It is also inhibited potently by two cancer-associated cellular proteins, I1PP2A and I2PP2A/SET. In addition, the SV40 small t antigen replaces the B subunit of PP2A during viral transformation. This subverts the physiological function of a subset of PP2A complexes in a substrate selective manner.

Figure: Purified preparation of bovine kidney PP2A2 was subjected to SDS-PAGE. The gel was stained with Coomassie Blue. The 65-kda A (top) and 36-kDa C (bottom) subunits are seen.

Protein Phosphatase 2A2 (PP2A2) is a dimeric form of PP2A. It contains A (65 kDa) and C (36 kDa) subunits but lacks the B subunit present in PP2A1. GloboZymes purified PP2A2 preparations are used to study enzyme kinetics and regulation. They are used to dephosphorylate target substrates and to evaluate the effects of test substances on the activity of the phosphatase. The preparations can also be used for determining the role of the missing B subunit of the enzyme.

References: Biochem J 287: 1019; Proc Natl Acad Sci USA 90: 2500

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。