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XNAP2E

Extract-N-Amp^™植物PCR试剂盒

Name: Extract-N-Amp<SUP>™</SUP>植物PCR试剂盒
Brand: SIGMA

sufficient for 100 extractions, sufficient for 500 amplifications

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别名:

Plant direct PCR kit

UNSPSC代码:

41106303

NACRES:

NA.55

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用途

sufficient for 100 extractions
sufficient for 500 amplifications
sufficient for 500 reactions

质量水平

200

特点

dNTPs included
hotstart

技术

PCR: suitable

颜色

colorless

运输

wet ice

储存温度

−20°C

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一般描述

Extract-N-Amp^™植物PCR试剂盒用于直接PCR（聚合酶链反应）。该试剂盒提供了从植物叶片快速提取基因组DNA以及通过PCR扩增靶标所需的所有试剂。它是一种创新的提取解决方案，无需常规的植物组织冷冻处理。

The PCR reaction mix facilitates amplification directly from the extract by using an antibody-based hot-start DNA polymerase for specific amplification.

应用

Extract-N-Amp^™植物PCR试剂盒适用于基因分型。

它已被用于从新鲜蘑菇中提取DNA。

Extract-N-Amp^™ Plant PCR Kit has been used to extract plant genomic DNA and in polymerase chain reaction (PCR).

特点和优势

PCR用植物基因组DNA可以在15分钟内提取。
无需冷冻、机械破碎、有机溶剂萃取、柱纯化或沉淀
经过特别配制的PCR ReadyMix 和提取的DNA一起使用
热启动抗体确保基因组DNA的高度特异性PCR扩增
适用于高通量植物基因分析
无需长时间的酶消化，节省时间和精力
提取的DNA在4 °C 下至少6个月保持稳定。

组分

Extract-N-Amp^™植物PCR试剂盒包括稀释溶液、提取溶液和Extract-N-Amp PCR 反应混合物（2X）（缓冲液、盐、dNTP、Taq聚合酶和JumpStart Taq抗体）。

Extraction Solution- E7526-12 mL

Dilution Solution- D5688-12mL

Extract-N-Amp PCR ReadyMix. This 2X PCR reaction mix contains buffer, salts, dNTPs, Taq polymerase, and JumpStart Taq antibody.- E3004- 5 x 1.2 ml

Collection tubes

其他说明

Extract-N-Amp植物PCR试剂盒仅供实验室使用。不可用于药物、家庭或其他用途。

The Extract-N-Amp^™ Plant PCR Kits are for laboratory use only. Not for drug, household, or other uses.

For additional information, please see www.sigma-aldrich.com/extract-n-amp.

法律信息

Extract-N-Amp is a trademark of Sigma-Aldrich Co. LLC

ReadyMix is a trademark of Sigma-Aldrich Co. LLC

WGK

WGK 3

闪点(°F)

Not applicable

闪点(°C)

Not applicable

法规信息

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Faster evolution of highly conserved DNA in tropical plants.

Len N Gillman et al.

Journal of evolutionary biology, 23(6), 1327-1330 (2010-05-12)

A faster rate of nuclear DNA evolution has recently been found for plants occupying warmer low latitudes relative to those in cooler high latitudes. That earlier study by our research group compared substitution rates within the variable internal transcribed spacer

Detection of Xanthomonas fragariae and presumptive detection of Xanthomonas arboricola pv. fragariae, from strawberry leaves, by real-time PCR.

S A Weller et al.

Journal of microbiological methods, 70(2), 379-383 (2007-06-26)

Real-time (TaqMan) PCR assays were developed to detect the strawberry angular leaf spot pathogen Xanthomonas fragariae (Xf) and the strawberry bacterial blight pathogen Xanthomonas arboricola pv. fragariae (Xaf). The Xf PCR (Xf gyrB) was designed within regions of the gyraseB

Signaling by the pathogenicity-related MAP kinase of Cochliobolus heterostrophus correlates with its local accumulation rather than phosphorylation.

Sophie Lev et al.

Molecular plant-microbe interactions : MPMI, 22(9), 1093-1103 (2009-08-07)

Phosphorylated mitogen-activated protein kinases (MAPK) transmit signals by activation of their targets. The extent of signal transduction could depend on MAPK phosphorylation level, concentration, and subcellular localization. The pathogenicity MAPK Chk1 of the fungal corn pathogen Cochliobolus heterostrophus is required

Melanin biosynthesis in the maize pathogen Cochliobolus heterostrophus depends on two mitogen-activated protein kinases, Chk1 and Mps1, and the transcription factor Cmr1.

Noa Eliahu et al.

Eukaryotic cell, 6(3), 421-429 (2007-01-24)

The maize pathogen Cochliobolus heterostrophus requires two mitogen-activated protein kinases (MAPKs), Chk1 and Mps1, to produce normal pigmentation. Young colonies of mps1 and chk1 deletion mutants have a white and autolytic appearance, which was partially rescued by a hyperosmotic environment.

A direct PCR approach to accelerate analyses of human-associated microbial communities.

Gilberto E Flores et al.

PloS one, 7(9), e44563-e44563 (2012-09-11)

Since the composition of the human microbiome is highly variable both within and between individuals, researchers are increasingly reliant on high-throughput molecular approaches to identify linkages between the composition of these communities and human health. While new sequencing technologies have

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商品

Extract-N-Amp™ Plant PCR Kits

Extract-N-Amp kits extract and amplify genomic DNA, optimized for plant tissue without inhibition concerns.

Extract-N-Amp™ Product Guide

Extract-N-Amp™ PCR kits are the world’s first integrated extraction and amplification process for rapid blood, tissue or plant assays.

基因组DNA样品纯化和质量评估

简单的DNA和RNA纯法方法大幅推动了基因组和基因表达的分析和鉴定。人们需要快速、方便地从多种细胞来源分离DNA和RNA，包括哺乳动物、植物和细菌培养物来源的细胞和组织。

Genomic DNA Purification and Assessment

Simple DNA/RNA purification methods aid genome analysis from various sources, enhancing research efficiency.

实验方案

Extract-N-Amp™ Plant PCR Kits Protocol

The Extract-N-Amp™ Plant PCR Kits contain all of the reagents required to rapidly extract and amplify genomic DNA from plant leaves.

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Extract-N-Amp™植物PCR试剂盒

sufficient for 100 extractions, sufficient for 500 amplifications

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Extract-N-Amp^™植物PCR试剂盒