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SIGMA 450243-10G 正钒酸钠 13721-39

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  • ¥775
  • Sigma-Aldrich
  • 进口
  • 450243-10G
  • 2025年10月30日
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    • 详细信息
    • 文献和实验
    • 技术资料
    • 保存条件

      常温

    • 保质期

      根据瓶身LOT号查询

    • 英文名

      Sodium orthovanadate

    • 库存

      有现货

    • 供应商

      浙江羽翔生物科技有限公司

    • CAS号

      13721-39-6

    • 规格

      10G

    属性

    产品名称

    正钒酸钠, 99.98% trace metals basis

    质量水平

    200

    方案

    99.98% trace metals basis

    表单

    solid

    反应适用性

    core: vanadium
    reagent type: catalyst

    mp

    850-866 °C (lit.)

    SMILES字符串

    [Na+].[Na+].[Na+].[O-][V]([O-])([O-])=O

    InChI

    1S/3Na.4O.V/q3*+1;;3*-1;

    InChI key

    IHIXIJGXTJIKRB-UHFFFAOYSA-N

    应用

    原钒酸钠(Na3VO4)可以用作以下合成反应的金属前体:
    • 阴离子交换法合成钒-MCM-48 (V-MCM-48)。V-MCM-48用作苯乙烯氧化为苯甲醛的催化剂。
    • 糖热法纳米化氧化钒颗粒。
    • 掺杂胶质铕的钒酸钇(YVO4)。

    生化/生理作用

    一种蛋白酪氨酸磷酸酶、碱性磷酸酶和ATP酶的抑制剂。
    抑制 ATP 酶、碱性磷酸酶和酪氨酸磷酸酶。在酸性 PH 值下形成的十钒酸盐可抑制肌醇基 1,4,5-三磷酸 (IP3)-诱导 Ca2+ 从内分泌细胞中的释放以及阻止 IP3 与其受体在脑组织中的结合。

    包装

    展示人体内的各种生物及生理效应。

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    图标文献和实验
    该产品被引用文献

    Temporal Dissection of Rate Limiting Transcriptional Events Using Pol II ChIP and RNA Analysis of Adrenergic Stress Gene Activation.

    PloS one (2015-08-06)
    Daniel P Morris, Beilei Lei, Lawrence D Longo, Karol Bomsztyk, Debra A Schwinn, Gregory A Michelotti
    PMID26244980
    摘要

    In mammals, increasing evidence supports mechanisms of co-transcriptional gene regulation and the generality of genetic control subsequent to RNA polymerase II (Pol II) recruitment. In this report, we use Pol II Chromatin Immunoprecipitation to investigate relationships between the mechanistic events controlling immediate early gene (IEG) activation following stimulation of the α1a-Adrenergic Receptor expressed in rat-1 fibroblasts. We validate our Pol II ChIP assay by comparison to major transcriptional events assessable by microarray and PCR analysis of precursor and mature mRNA. Temporal analysis of Pol II density suggests that reduced proximal pausing often enhances gene expression and was essential for Nr4a3 expression. Nevertheless, for Nr4a3 and several other genes, proximal pausing delayed the time required for initiation of productive elongation, consistent with a role in ensuring transcriptional fidelity. Arrival of Pol II at the 3' cleavage site usually correlated with increased polyadenylated mRNA; however, for Nfil3 and probably Gprc5a expression was delayed and accompanied by apparent pre-mRNA degradation. Intragenic pausing not associated with polyadenylation was also found to regulate and delay Gprc5a expression. Temporal analysis of Nr4a3, Dusp5 and Nfil3 shows that transcription of native IEG genes can proceed at velocities of 3.5 to 4 kilobases/min immediately after activation. Of note, all of the genes studied here also used increased Pol II recruitment as an important regulator of expression. Nevertheless, the generality of co-transcriptional regulation during IEG activation suggests temporal and integrated analysis will often be necessary to distinguish causative from potential rate limiting mechanisms.

    相关实验
    • 3'-RACE PCR

      steps c. - e. 35 times      g. 72°C 10 minutes.   * Varies according to the melting temperature of your gene specific primer. The annealing temperature in the PCR may require some adjustment for optimal yield of PCR product.  

    • 3'RACE PCR

      . - e. 35 times g. 72°C 10 minutes. * Varies according to the melting temperature of your gene specific primer. The annealing temperature in the PCR may require some adjustment for optimal yield of PCR product. 8. Load

    • Protocol for 5' End Labeling RNA

      实验步骤   1. Protocol for Removing 5' Phosphate 1) Combine the following in a single RNase-free microfuge tube: -- µl Nuclease-free Water (to make a final volume of 10 µl) -- µl RNA (0.1Ï10 pmol RNA) 1 µl

    图标技术资料

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    文献支持
    SIGMA 450243-10G 正钒酸钠 13721-39-6
    ¥775