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Merck

S9194

Sigma-Aldrich

高通量 QPCR 用 SYBR® Green JumpStart Taq ReadyMix

SYBR® Green qPCR reagent, passive reference dye included

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About This Item

分類程式碼代碼:
41106300
NACRES:
NA.55

品質等級

形狀

liquid

用途

sufficient for 20 reactions
sufficient for 2000 reactions
sufficient for 400 reactions

特點

dNTPs included
hotstart

濃度

1.25 units/reaction (50 μL reaction volume)

技術

qPCR: suitable

顏色

colorless

輸入

purified DNA

相容性

for use with ABI 5700
for use with ABI 7000
for use with ABI 7300
for use with ABI 7700
for use with ABI 7900 Fast
for use with ABI 7900 HT
for use with ABI 7900
for use with ABI StepOne
for use with ABI StepOnePlus

檢測方法

SYBR® Green

運輸包裝

wet ice

儲存溫度

−20°C

一般說明

SYBR® Green JumpStart Taq ReadyMix is a ready-to-use 2X master mix that contains SYBR® Green I, JumpStart Taq DNA polymerase, 99% pure deoxynucleotides (dNTPs), and reaction buffer making it the ideal solution for performing high-throughput quantitative PCR. SYBR® Green I dye binds to and detects any dsDNA generated during amplification. The JumpStart Taq DNA polymerase is an antibody-inactivated hot-start enzyme. Once the reaction temperature reaches 70°C, the DNA polymerase-antibody complex dissociates and Taq DNA polymerase activity is restored. This antibody-enzyme complex allows for easy and convenient set-up with less contamination risk than manual hot-start techniques.

應用

SYBR® Green JumpStart Taq ReadyMix for High Throughput qPCR has been used for the amplification and quantification of transcripts to analyze gene expression in 2-step quantitative reverse transcription PCR (RT-qPCR). It has also been used for quantitative polymerase chain reaction (qPCR) of reverse-transcribed cDNA.

特點和優勢

  • The master mix allows consistency and reproducibility from one reaction to the next
  • Reduced set-up time as compared to manual or wax Hot Start methods
  • Reduced primer dimers
  • Allows for room temperature set-up; Ideal for high throughput, quantitative PCR application
  • SYBR® Green I dye binds to double-stranded DNA and is ideal for quantifying any DNA sequence. Detection is monitored by measuring the increase in fluorescence throughout cycling.
  • JumpStart Taq DNA polymerase prevents amplification of non-specific products while increasing target yield.
  • Internal Reference Dye is provided for reaction normalization. Maximum excitation and emission is 586 nm and 605 nm, respectively.
  • SYBR Green JumpStart Taq ReadyMix reduces preparation time and the risk of contamination from multiple pipetting steps.

包裝

Default reaction volume is 50 μL

20RXN is packaged as 1 X 500 μL
400RXN is packaged as 1 X 10 mL
2000RXN is packaged as 1 X 50 mL

其他說明

SYBR Green ReadyMix for High Throughput Quantitative PCR combines the performance enhancements of JumpStart Taq and SYBR Green I in an easy-to-use ReadyMix solution that incorporates ROX dye for ABI and other real time instrument applications. The ReadyMix includes a detection fluor, internal standard and reagents for PCR making it the ideal solution for performing high-throughput quantitative PCR.

法律資訊

本品的使用受以下一个或多个美国专利和美国之外相应专利权利要求的保护:5,079,352、5,789,224、5,618,711、6,127,155、5,677,152(仅权利要求 1 至 23 项)、5,773,258(仅权利要求 1 和 6 项)、5,407,800、5,322,770、5,310,652、5,994,056、6,171,785,以及受对应于美国专利4,889,818 的美国之外的权利要求的保护。受前述专利权利要求的保护,本品的购买包括有限的、不可转让的豁免权,只可将该数量的产品用于购买者自己的内部研究。未通过暗示、默许明确让与任何其他专利权利要求(例如美国专利6,814,934 中的设备或系统权利要求)下的权利,以及进行任何商业服务的权利,包括但不限于出于有偿或其他商业考虑而报道购买者的实验结果。本品只可用于研究目的。受 Roche 专利保护的诊断用途需要获得 Roche 的单独许可。关于购买许可的更多信息,请联系许可总监 (Applied Biosystems, 850 Lincoln Centre Drive, Foster City, California 94404, USA)。
JumpStart is a trademark of Sigma-Aldrich Co. LLC
ReadyMix is a trademark of Sigma-Aldrich Co. LLC
SYBR is a registered trademark of Life Technologies

象形圖

Exclamation markEnvironment

訊號詞

Warning

危險分類

Aquatic Chronic 2 - Eye Irrit. 2 - Skin Irrit. 2 - Skin Sens. 1

儲存類別代碼

10 - Combustible liquids

水污染物質分類(WGK)

WGK 3


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访问文档库

Gene resistance to transcriptional reprogramming following nuclear transfer is directly mediated by multiple chromatin-repressive pathways
<BIG><BIG>Jullien J, et al.</BIG></BIG>
Molecular Cell, 873-884 (2017)
Fank1 and Jazf1 promote multiciliated cell differentiation in the mouse airway epithelium
<BIG><BIG>Johnson JA, et al.</BIG></BIG>
Biology Open, 7, bio033944-bio033944 (2018)
Narcisa Muresu et al.
Virology journal, 17(1), 161-161 (2020-10-24)
Human Papillomavirus (HPV) infection is one of the most important causes of cancer. It can play a role in cervical and extra-cervical cancers. Penile cancer is rare, even if an increasing trend was recently reported. Aim of the present study
Narcisa Muresu et al.
International journal of environmental research and public health, 17(12) (2020-06-27)
Objectives: Anal cancer is a rare disease. However, its incidence is increasing in some population groups. Infection caused by Human Papillomavirus (HPV) is strongly associated with the risk of anal cancer, whose variability depends on samples, histology, and HPV detection
Sambrook, J., and Russell, D.W.
Molecular Cloning: A Laboratory Manual null

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实验方案

A protocol that can be used as a basic template for qPCR incorporating SYBR Green I DNA binding dye that is amenable to modification and applicable for use as validation for a set of primers.

A protocol that can be used as a basic template for qPCR incorporating SYBR Green I DNA binding dye that is amenable to modification and applicable for use as validation for a set of primers.

A protocol that can be used as a basic template for qPCR incorporating SYBR Green I DNA binding dye that is amenable to modification and applicable for use as validation for a set of primers.

A protocol that can be used as a basic template for qPCR incorporating SYBR Green I DNA binding dye that is amenable to modification and applicable for use as validation for a set of primers.

相关内容

SYBR® Green I, a commonly used fluorescent DNA binding dye, binds all double-stranded DNA and detection is monitored by measuring the increase in fluorescence throughout the cycle. Explore our LuminoCt® and KiCqStart® products for Fast qPCR or JumpStart™ reagents for conventional qPCR

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