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RAB0308

Sigma-Aldrich

小鼠 IL-6 ELISA 试剂盒

for serum, plasma and cell culture supernatant

别名:

B-cell stimulatory factor 2, CTL differentiation factor, Hybridoma growth factor, IFN-beta-2, IL-6, Interferon beta-2

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1 KIT
$858.00

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1 KIT
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About This Item

分類程式碼代碼:
41116158
NACRES:
NA.84

$858.00


请联系客服了解存货情况

物種活性

mouse

包裝

kit of 96 wells (12 strips x 8 wells)

技術

ELISA: suitable
capture ELISA: suitable

輸入

sample type plasma
sample type cell culture supernatant(s)
sample type serum

assay range

inter-assay cv: <12%
intra-assay cv: <10%
sensitivity: 2 pg/mL
standard curve range: 0.82-600 pg/mL

檢測方法

colorimetric

運輸包裝

wet ice

儲存溫度

−20°C

基因資訊

mouse ... Il6(24498)

一般說明

小鼠 IL-6 ELISA(酶联免疫吸附试验)试剂盒是一种体外酶联免疫吸附试验,用于定量测定血清、血浆、细胞培养上清液和尿液中的小鼠 IL-6。

免疫原

重组小鼠 IL-6

應用

仅用于研究目的。不用于诊断程序。
小鼠白介素 6 (IL-6) ELISA 试剂盒用于测定生物样品中 IL-6 的含量。[1][2][3]

生化/生理作用

IL-6 是一种多效性细胞因子,通过调节免疫和炎症反应在宿主防御中发挥重要作用。IL-6 由 T 细胞、单核细胞、成纤维细胞、内皮细胞和角质形成细胞产生,具有多种生物学功能。刺激 B 细胞分化和抗体生成,与 IL-3 协同作用于巨核细胞发育和血小板生成,诱导肝脏急性期蛋白表达,调节骨代谢。[4]

其他說明

本产品提供样品分析证书。
请在批号文本框中输入汉字 样本

试剂盒组分也可单独购买

产品编号
说明
化学品安全说明书

  • RABELADBELISA 5X Assay/Sample Diluent Buffer B (Item E1)化学品安全说明书

  • RABSTOP3ELISA Stop Solution (Item I)化学品安全说明书

  • RABTMB3ELISA Colorimetric TMB Reagent (HRP Substrate, Item H)化学品安全说明书

  • RABWASH420X Wash Buffer (Item B)化学品安全说明书

象形圖

Corrosion

訊號詞

Warning

危險聲明

防範說明

危險分類

Met. Corr. 1

儲存類別代碼

8A - Combustible corrosive hazardous materials


历史批次信息供参考:

分析证书(COA)

Lot/Batch Number

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The biology of interleukin-6.
Kishimoto T
Blood, 74(1), 1-10 (1989)
Effect of HI-6 on cytokines production after immunity stimulation by keyhole limpet hemocyanin in a mouse model.
Pohanka M
Neuro Endocrinology Letters, 35, 155-157 (2014)
Cytocompatible Anti-microbial Dressings of Syzygium cumini Cellulose Nanocrystals Decorated with Silver Nanoparticles Accelerate Acute and Diabetic Wound Healing.
Singla R
Scientific Reports, 7(1), 10457-10457 (2017)
Rubbel Singla et al.
Scientific reports, 7(1), 10457-10457 (2017-09-07)
The ever increasing incidences of non-healing skin wounds have paved way for many efforts on the convoluted process of wound healing. Unfortunately, the lack of relevance and success of modern wound dressings in healing of acute and diabetic wounds still
Laura N Castellani et al.
Scientific reports, 8(1), 772-772 (2018-01-18)
Olanzapine is a widely prescribed antipsychotic drug. While effective in reducing psychoses, treatment with olanzapine causes rapid increases in blood glucose. We wanted to determine if a single bout of exercise, immediately prior to treatment, would attenuate the olanzapine-induced rise

Questions

1–2 of 2 Questions  
  1. Hello. How much should I dilute tissue culture media for the assay? 2-fold? Thanks.

    1 answer
    1. The Assay/Sample Diluent Buffer (Item E2) should be diluted 5-fold. This 1X Assay/Sample Diluent Buffer is used to dilute serum, plasma, or medium samples a recommended 2 fold. Please note that the levels of IL-6 may vary between different samples. Optimal dilution factors for each sample must be determined by the investigator.

      Helpful?

  2. マウスのパイエル板をホモジナイズした上清で測定は可能ですか?

    1 answer
    1. This product is suitable with serum, plasma, and cell culture supernatant. However, it has not been determined if this product can measure the supernatant obtained by homogenizing mouse Peyer's patches. This application will need to be validated by the end-user.

      While the requested ELISA kit nor any of the offered normal ELISA kits are neither designed nor validated with cell/tissue lysate samples, our kits are very accommodating to many different sample types so lysates will most likely work. If it is decided to test these kits with cell/tissue lysate samples, it is recommended to dilute the samples at least 5-fold with Assay Diluent to minimize any effects of the detergents in the lysis buffer. The samples may need to be diluted further but this would need to be determined by the experimenter empirically.

      So for the original lysate, in general it is recommended to shoot for at least 1 mg/ml protein, preferably more, to achieve 50-500 ug/ml after dilution. Again though, this range should just be used as a starting point and the optimal concentration would need to be determined empirically.

      Below are some general guidelines for doing so along with some basic tips for sample preparation.
      Tips on Sample preparation
      In brief, a lysis buffer must meet the following specifications:
      A) has relatively low salt content (700 mM or less)
      B) does not contain sodium azide
      C) does not contain >0.1% SDS
      D) does not contain >10 mM reducing agents (beta-mercaptoethanol or dithiothreitol)
      This would include any buffers used for immunoprecipitations, including RIPA buffer.

      Helpful?

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