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  m6A RNA甲基化文库构建试剂盒(测序版) (A-P-9016)
   

m6A RNA甲基化文库构建试剂盒(测序版)                                货号:A-P-9016

EpiNext CUT&RUN RNA m6A-Seq Kit 

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背景资料:N6-methyladenosine (m6A) is the most common and abundant modification on RNA molecules present in eukaryotes. Recently, DNA m6A is also identified in multicellular eukaryotes including Caenorhabditis elegans and Drosophila melanogaster, and furthermore identified in higher eukaryotes including plants, mouse and human cells. m6A plays crucial roles in regulating DNA replication, DNA damage, RNA splicing, transposition, transcription, and cellular defense. In human cells, the m6A modification is probably catalyzed by a methyltransferase complex METTL3/METTL14 and removed by the α-ketoglutarate (α-KG)- and Fe2+-dependent dioxygenases such as FTO, ALKBH5 and TET-like enzymes. It was shown that METTL3 and α-KG /Fe2+-dependent dioxygenases play important roles in many biological processes, ranging from development and metabolism to fertility. The dynamic and reversible chemical m6A modification on DNA /RNA may also serve as a novel epigenetic marker of profound biological significance. Down-regulation of m6A modification was first characterized in human cancer cells and tissues, relative to their normal controls. m6A is found to be the most regulated DNA modification in cancers. In addition to the regulation in cancer cells, relative to the primary cell/tissues which contain quite low DNA m6A (<0.001%), a hundreds-fold increase of m6A modification was found for in vitro cultured human cells (0.03%-0.22%)

产品描述:This kit is designed for measuring total m6A demethylase activity/inhibition. In an assay with this kit, the unique m6A substrate is stably coated on the strip wells. Active m6A demethylases bind to and demethylate m6A contained in the substrate. The un-demethylated m6A in the substrate can be recognized with a high affinity m6A antibody and the immuno-signal is enhanced with enhancer solution. The ratio or amount of un-demethylated m6A, which is inversely proportional to enzyme activity, can then be colorimetrically quantified through an ELISA-like reaction

产品特点:

High enrichment: Use RNA cleavage enzyme mix to simultaneously fragment RNA and cleave/remove any RNA sequences at both ends of the target m6A -containing sequences without affecting RNA regions occupied by the antibody. Short RNA fragments are generated only bound with anti- m6A antibody. True target m6A-enriched regions can, therefore, be reliably identified and high-resolution mapping achieved

Low Input: Unbound RNA cleavage and immunocapture are processed in the same single-tube, which enables the maximal protection of the target m6A-containing regions and the minimized sample loss, allowing the input RNA to be as low as 500 ng

3.Minimal Background: Cleavage of unbound RNA sequences in the two ends of the target m6A-containing sequences enables the minimized MeRIP/sequencing background, allowing data analysis with <10 million reads.
4.Fast, streamlined procedure: The procedure from RNA to library cDNA is less than 6 hours with <1 h of hands-on time

5.Highly convenient: The kit contains all required components for each step of the CUT&RUN RNA m6A -Seq, which are sufficient for both m6A-containing RNA sequence capture and captured cDNA library preparation, thereby allowing CUT&RUN RNA m6A –Seq to be the most convenient with reliable and consistent results

数据分析: 

操作流程 标准曲线
EpiNext m6A RNA甲基化文库构建试剂盒(测序版) 流程图 Size distribution of library fragments. m6Afragments were enriched from 3 ug of total RNA by the anti- m6A antibody (EpiGentek, #A-1801) and used for cDNA library preparation. Peak at 195 bps reflects insert


参考文献:

1.Lewinska A et. al. (February 2017). Downregulation of Methyltransferase Dnmt2 Results in Condition-dependent Telomere Shortening and Senescence or Apoptosis in Mouse Fibroblasts. J Cell Physiol.

保存建议:在接收到艾德寄出的试剂盒后请按照说明书建议,使用不同的保存条件或温度来保存试剂盒内组分。

定购信息:    
产品名称 规格 操作手册 货号 询价
m6A RNA甲基化文库构建试剂盒(测序版)  24次 中文PDF A-P-9016-24 点击这里给我发消息
m6A RNA甲基化文库构建试剂盒(测序版)  12次 中文PDF A-P-9016-12  
m6A去甲基化酶活性/抑制分析试剂盒(比色法) 96次 英文PDF-中文PDF A-P-9013-96 点击这里给我发消息
m6A去甲基化酶活性/抑制分析试剂盒(比色法) 48次 英文PDF-中文PDF A-P-9013-48  
m6A RNA甲基化定量检测试剂盒(荧光法) 96次 英文PDF-中文PDF A-P-9008-96 点击这里给我发消息
m6A RNA甲基化定量检测试剂盒(荧光法) 48次 英文PDF-中文PDF A-P-9008-48  
尿液样本 m6A RNA甲基化定量检测试剂盒(比色法) 96次 英文PDF-中文PDF A-P-9015-96 点击这里给我发消息
尿液样本 m6A RNA甲基化定量检测试剂盒(比色法) 48次 英文PDF-中文PDF A-P-9015-48  
总体RNA甲基化极易定量检测试剂盒(荧光法) 96次 英文PDF-中文PDF A-P-9009-96 点击这里给我发消息
总体RNA甲基化极易定量检测试剂盒(荧光法) 48次 英文PDF-中文PDF A-P-9009-48  
总组蛋白H3K27乙酰化定量检测试剂盒(比色法) 48次 PDF A-P-4059-48  
总组蛋白H3K27乙酰化定量检测试剂盒(比色法) 96次 PDF A-P-4059-96  
EpiNext 高灵敏重亚硫酸盐测序试剂盒(Illumina) 12次 PDF A-P-1056A-12
EpiNext 高灵敏重亚硫酸盐测序试剂盒(Illumina) 24次 PDF A-P-1056A-24 点击这里给我发消息
96孔DNA甲基化极速修饰试剂盒(磁珠法)  96次 英文PDF-中文PDF A-P-1050-096  
96孔DNA甲基化极速修饰试剂盒(磁珠法)  192次 英文PDF-中文PDF A-P-1050-192  
抗人C5a/C5a desArg单克隆抗体(克隆号2942) 100ug C-HM2078  
抗人TNF-R II单克隆抗体(克隆号80M2),FITC标记 100ug C-HM2022F  
抗人TNF-R II单克隆抗体(克隆号MR2-1),生物素标记 50ug C-HM2008  
抗人TNF-R I单克隆抗体(克隆号MR1-2),生物素标记 50ug C-HM2006  
抗小鼠TREM-2单克隆抗体(克隆号6E9) 100ug PDF  C-HM1129F 点击这里给我发消息
m6A RNA甲基化定量检测试剂盒(比色法) 96 次 英文PDF--中文PDF A-P-9005-96  
RNA甲基化修饰试剂盒 50 次 英文PDF--中文PDF A-P-9003-050  
EZ RNA甲基化修饰试剂盒 50 次 英文PDF--中文PDF A-R5001  

表观遗传学产品全面解决方案列下:   

产品名称 规格 操作手册 货号 询价
DNA羟甲基化定量试剂盒(比色法) 48 次 英文PDF--中文PDF A-P-1036-48 点击这里给我发消息
DNA羟甲基化定量试剂盒(比色法) 96 次 英文PDF--中文PDF A-P-1036-96  
DNA羟甲基化定量试剂盒(荧光法) 48 次 英文PDF--中文PDF A-P-1037-48 点击这里给我发消息
DNA羟甲基化定量试剂盒(荧光法) 96 次 英文PDF--中文PDF A-P-1037-96  
DNA甲基化定量试剂盒(荧光法) 48 次 英文PDF--中文PDF A-P-1035-48 点击这里给我发消息
DNA甲基化定量试剂盒(荧光法) 96 次 英文PDF--中文PDF A-P-1035-96  
DNA甲基化定量试剂盒(比色法) 48 次 英文PDF--中文PDF A-P-1034-48 点击这里给我发消息
DNA甲基化定量试剂盒(比色法) 96 次 英文PDF--中文PDF A-P-1034-96  
总体DNA甲基化极易定量试剂盒(比色法) 48 次 英文PDF--中文PDF A-P-1030-48 点击这里给我发消息
总体DNA甲基化极易定量试剂盒(比色法) 96 次 英文PDF--中文PDF A-P-1030-96  
总体DNA羟甲基化极易定量试剂盒(比色法) 48 次 英文PDF--中文PDF A-P-1032-48 点击这里给我发消息
总体DNA羟甲基化极易定量试剂盒(比色法) 96 次 英文PDF--中文PDF A-P-1032-96  
总DNA甲基化定量试剂盒 48 次 英文PDF--中文PDF A-P-1014B-48 点击这里给我发消息
总DNA甲基化定量试剂盒 96 次 英文PDF--中文PDF A-P-1014B-96  

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关于5-hmC
5-hmC是近年来在动物组织中发现的,由胞嘧啶修饰而来。5-hmC在表观遗传学上的功能可能与5-甲基化胞嘧啶(5-mC)不同。尽管到现在为止还不确知其功能,有研究者猜测它在调控基因的表达与关闭过程中起着重要的作用。5-mC的发现让我们不得不重新评估DNA甲基信息,也不得不监测人类的健康组织和病理组织之间5-mC相对分布的差异。在EPI公司的MethylFlash技术之前,我们还没有发现任何直接的常规方法来检测5- hmC,以及区分5-hmC和5-mC

5-hmC 和 5-mC的区别

时下常用的DNA甲基化分析方法包括限制内切酶酶切和亚硫酸氢盐或MeDIP介导的MS-PCR和测序,这些技术都不适合用来检测5-hmC,因为它与5-mC事实上很难用这类方法区分开来。为了解决这个问题,EPIk研制了MethylFlash羟甲基化DNA定量试剂盒(荧光法)。本试剂盒提供了一种很经济的方法来检测5-羟甲基化胞嘧啶,并且区分5-hmC, 5-mC, 和 C,使得研究者能够重新评估他们的DNA甲基化信息,也能够在新样品中寻找DNA羟甲基化。

 
 
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