TGIRT™-III Enzyme
規(guī)格:
10 Reactions (TGIRT10)
50 Reactions (TGIRT50)
5 x 50 µl (TGIRT5x50)
10 x 50 µl (TGIRT10x50)
單位定義:
TGIRT的一個(gè)單元® -III逆轉(zhuǎn)錄酶(RT)活性是酶的使用聚在60℃下聚合1納摩爾的dNTP的在1分鐘(RA)所需要的量/寡(dT)42作為底物��。
酶濃度:
200單位/μl
酶儲(chǔ)存緩沖液:
20mM Tris-HCl(pH 7.5),500mM KCl��,1mM EDTA����,1mM DTT,50%甘油
酶屬性和新穎活動(dòng):
比逆轉(zhuǎn)錄逆轉(zhuǎn)錄酶更高的熱穩(wěn)定性�����,持續(xù)合成能力和保真度��,允許從高度結(jié)構(gòu)化或重度修飾的RNA (例如tRNA)和包含富含GC的重復(fù)擴(kuò)增的RNA合成全長(zhǎng)�����,端對(duì)端cDNA ����。1-9,12,15,18
新型端對(duì)端模板轉(zhuǎn)換活動(dòng),可在反轉(zhuǎn)錄過程中連接RNA-seq或PCR適配器����,并且無(wú)需單獨(dú)的RNA 3'-適配器連接步驟�����。1這種模板轉(zhuǎn)換活性極大地促進(jìn)了鏈特異性RNA-seq文庫(kù)的構(gòu)建����,而且比使用隨機(jī)六聚體引物或使用RNA連接酶進(jìn)行銜接子連接的方法具有更小的偏差��。1,7,8
從退火引物合成cDNA����。將退火的引物應(yīng)具有推測(cè)的T 米 > 60的直徑: C.酶與反應(yīng)底物混合,在室溫下�����,通過加入dNTP的反應(yīng)開始30分鐘的預(yù)溫育��,建議����。新應(yīng)用的zui宜條件應(yīng)該通過測(cè)試25-450mM NaCl的一系列鹽濃度來(lái)確定。
建議用于酶的用途:
1.全面的鏈特異性轉(zhuǎn)錄組分析��。8
2.全細(xì)胞��,外泌體�����,血漿和其他無(wú)細(xì)胞RNA的RNA-seq����。7,8,15
3.分析miRNA,tRNA和其他小的非編碼RNA����。1-9,12,15
4. RIP-seq,HITS-CLIP��,irCLIP和CRAC用于表征RNA-蛋白質(zhì)相互作用和核糖體分析��。1,10,11
5.通過高通量測(cè)序鑒定RNA堿基修飾��。4,5,13,??14
6.使用諸如SHAPE和DMS修飾的方法進(jìn)行全基因組或靶向RNA結(jié)構(gòu)作圖����。1,16
7.富含GC重復(fù)擴(kuò)增的逆轉(zhuǎn)錄和定量。18
8.長(zhǎng)cDNA的合成����。1
9.RT-qPCR�����。1
10.單鏈DNA-seq����。17
11.分析FFPE腫瘤樣本(咨詢InGex)。
酶的優(yōu)點(diǎn):
1.全面的鏈特異性轉(zhuǎn)錄組分析��。
核糖核碎片�����,通用人類參考RNA樣品的TGIRT®-seq概括了人類轉(zhuǎn)錄物和穗突起的相對(duì)豐度��,與非鏈特異性TruSeq v2相比�����,并且優(yōu)于鏈特異性Tru-Seq v3。TGIRT®-seq比TruSeq v3具有更高的鏈特異性��,并消除了TruSeq固有的隨機(jī)六聚體引發(fā)的取樣偏差��。TGIRT®-seq顯示出更加統(tǒng)一的5'至3'基因覆蓋范圍�����,并且比TruSeq識(shí)別更多的剪接點(diǎn)��。TGIRT®-seq能夠在與結(jié)構(gòu)化小型ncRNA相同的RNA-seq中同時(shí)分析mRNA和lncRNA��,包括tRNA�����,TruSeq數(shù)據(jù)集基本上不存在tRNA�����。8
2.全細(xì)胞����,外泌體�����,血漿和其他細(xì)胞外RNA的RNA-seq����。
快速的處理時(shí)間(通過PCR步驟對(duì)RNA-seq文庫(kù)構(gòu)建<5小時(shí)); 需要少量的RNA(低ng范圍); 包括mRNA和lncRNA以及小ncRNA的全面轉(zhuǎn)錄譜�����,包括tRNA�����,pre-miRNA和其他結(jié)構(gòu)化小型ncRNA的全長(zhǎng)讀段; 比常規(guī)方法更少的偏差和更大的鏈特異性�����。7,8,15
3.通過TGIRT®模板轉(zhuǎn)換的RNA-seq文庫(kù)構(gòu)建,如RIP-seq����,HITS-CLIP,irCLIP�����,CRAC,??核糖體譜分析��。
快速的處理時(shí)間(通過PCR步驟對(duì)RNA-seq文庫(kù)構(gòu)建<5小時(shí)); 需要少量的RNA(低ng范圍); 不需要RNA連接酶����,通過減少步驟中的步驟來(lái)減少偏倚并提率。1,10,11
4.比逆轉(zhuǎn)錄病毒RT更高的熱穩(wěn)定性����,持續(xù)合成能力和鏈置換活性。
使用錨定寡核苷酸(dT)引物�����,可以構(gòu)建RNA聚合腺苷酸化的RNA文庫(kù)����,與沒有ribodepletion步驟的逆轉(zhuǎn)錄病毒RT相比,具有更均勻的5'至3'覆蓋范圍��。1
通過基于毛細(xì)管電泳的方法(如SHAPE或DMS結(jié)構(gòu)圖)進(jìn)行RNA結(jié)構(gòu)作圖��,其顯著的讀數(shù)長(zhǎng)度和更少的提前停止時(shí)間比逆轉(zhuǎn)錄病毒RTs更短�����。1,16
可以分析含有富含GC的重復(fù)擴(kuò)增的RNA模板。18
能夠合成來(lái)自tRNA和其他小型結(jié)構(gòu)化/修飾的ncRNA的全長(zhǎng)�����,端對(duì)端cDNA��,這些逆轉(zhuǎn)錄病毒RT難以治療��。4-9,12-15
5.人血漿和大腸桿菌 基因組DNA的ssDNA-seq ��。
通過直接在DNA鏈的3'末端啟動(dòng)DNA合成��,同時(shí)連接DNA-seq接頭而不進(jìn)行末端修復(fù)����,拖尾或連接�����,以更簡(jiǎn)單的工作流程捕獲的DNA末端�����。能夠分析核小體定位,轉(zhuǎn)錄因子結(jié)合位點(diǎn)����,DNA甲基化位點(diǎn)和起源組織。17
參考文獻(xiàn):
- Mohr, S., Ghanem, E., Smith, W., Sheeter, D., Qin, Y., King, O., Polioudakis, D., Iyer, V.R., Hunicke-Smith, S. Swamy, S., Kuersten, S., and Lambowitz, A.M. Thermostable group II intron reverse transcriptase fusion proteins and their use in cDNA synthesis and next-generation RNA sequencing. RNA 19, 958-970, 2013.
- Collins, K. and Nilsen, T. Enzyme engineering through evolution: thermostable recombinant group II intron reverse transcriptases provide new tools for RNA research and biotechnology. RNA 19, 1017-1018, 2013.
- Enyeart, P.J., Mohr, G., Ellington, A.D., and Lambowitz A.M. Biotechnological applications of group II introns and their reverse transcriptases: gene targeting, RNA-seq, and non-coding RNA analysis. DNA 5:2, 2014.
- Katibah, G.E., Qin, Y., Sidote, D.J., Yao, J., Lambowitz, A.M. and Collins, K. Broad and adaptable RNA structure recognition by the human interferon-induced tetratricopeptide repeat protein IFIT5. Proc. Natl. Acad. Sci., USA, 111, 12025-12030, 2014.
- Shen, P.S., Park, J., Qin, Y., Li, X., Parsawar, K., Larson, M.H., Cox, J., Chen, Y., Lambowitz, A.M., Weissman, J.S., Brandman, O., and Frost, A. Rqc2p and 60S ribosomal subunits mediate mRNA-independent elongation of nascent chains. Science 347, 75-78, 2015.
- Zheng, G., Qin, Y., Clark, W.C., Yi, C., He, C., and Lambowitz, A.M. and Pan, T. Efficient and quantitative high-throughput transfer RNA sequencing. Nat. Methods 12, 835-837, 2015.
- Qin,Y., Yao,J., Wu,D., Nottingham, R., Mohr, S, Hunicke-Smith, S., Lambowitz, A.M., High-throughput sequencing of human plasma RNA by using thermostable group II intron reverse transcriptases. RNA 22, 111-128, 2016.
- Nottingham, R.M., Wu, D.C., Qin, Y., Yao, J., Hunicke-Smith, S., and Lambowitz, A.M. RNA-seq of human reference RNA samples using a thermostable group II intron reverse transcriptase. RNA 22, 597-613, 2016.
- Burke, J.M., Kincaid, R.P., Nottingham, R.M., Lambowitz, A.M., and Sullivan, C.S. DUSP11 activity on tri-phosphorylated transcripts promotes Argonaute association with noncanonical viral microRNAs and regulates steady state levels of cellular non-coding RNAs. Genes & Dev. 30, 2071-2092, 2016.
- Zarnegar, B.J., Flynn, R.A., Shen, Y., Do, B.T., Chang, H.Y. and Khavari, P.A. irCLIP platform for characterization of protein-RNA interactions. Nat. Methods 13, 489-492, 2016.
- Haque, N. and Hogg, J.R. Easier, better, faster, stronger: Improved methods for RNA-protein interaction studies, Mol. Cell, 2016 http//dx.doi.org/10.1016/j.molcel.2016.05.019
- Bazzini, A.A., del Viso, F., Moreno-Mateos, M.A., Johnstone, T.G., Vejnar, C.E., Qin, Y., Yao, J., Khokha, M.K., and Giraldez, A.J. Codon identity regulates mRNA stability and translation efficiency during the maternal-to-zygotic transition. EMBO J. 35, 2087-2103, 2016.
- Clark, W.C., Evans, M.E., Dominissini, D., Zheng, G., and Pan, T. tRNA base methylation identification and quantification via high-throughput sequencing. RNA 22, 1771-1784, 2016.
- Liu et al. ALKBH-mediated tRNA demethylation regulates translation. Cell 167, 816-828, 2016,
- Shurtleff, M.J., Yao, J., Qin, Y., Nottingham, R.M., Temoche-Diaz, M., Schekman, R., and Lambowitz, A.M. A broad role for YBX1 in defining the small non-coding RNA composition of exosomes. Proc. Natl. Acad. Sci. U.S.A. 114, 8987-8995, 2017.
- Zubradt, M., Gupta, P., Persad, S., Lambowitz, A.M., Weissman, J.S., and Rouskin, S. DMS-MaPseq for genome-wide or targeted RNA structure probing in vivo. Nature Methods 10.1038/nmeth.4057, 2016.
- Wu, D.C., and Lambowitz, A.M. Facile single-stranded DNA sequencing of human plasma DNA via thermostable group II intron reverse transcriptase template switching. Scientific Reports 7, 8421, 2017.
- Carrell, S.T., Tang, Z., Mohr, S., Lambowitz, A.M, and Thorton, C.A. Detection of expanded RNA repeats using thermostable group II intron reverse transcriptase. Nucleic Acids Res. 46, e1, 2018.
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