标签归档:dutp

5-Propargylamino-3′-azidomethyl-dUTP 货号17093-AAT Bioquest荧光染料

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上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

5-Propargylamino-3′-azidomethyl-dUTP

5-Propargylamino-3′-azidomethyl-dUTP

5-Propargylamino-3'-azidomethyl-dUTP 货号17093 货号 17093 存储条件 在零下15度以下保存, 避免光照
规格 50 nmoles 价格 3108
Ex (nm) Em (nm)
分子量 576.24 溶剂 Water
产品详细介绍

简要概述

产品基本信息

货号:17093

产品名称:5-Propargylamino-3′-azidomethyl-dUTP

规格:50 nmoles

储存条件:-15℃避光防潮

保质期:24个月

 

产品物理化学光谱特性

分子量:576.24

溶剂:水

 

产品介绍

5-Propargylamino-3′-azidomethyl-dUTP是制备用于下一代测序(NGS)的荧光缀合物的关键组成部分。 NGS使用与早期Sanger测序相似的链终止方法,但NGS是通过荧光标记的核苷酸类似物作为扩增反应的可逆终止剂来进行的。 NGS依赖于可逆的DNA聚合阻断,而Sanger测序则使用ddNTP不可逆转的DNA聚合阻断。 NGS的另一个不同特征是通过桥式PCR进行体外克隆扩增以增加待测序分子的数量。在此平台上,片段与固定在固体表面上的引物连接,进行原位扩增,生成具有相同分子的DNA簇。在每个循环中,同时添加可逆终止的四个核苷酸,并通过它们互补的聚合酶掺入。通过将3′-OH基团替换为3′-o-叠氮基甲基,这些核苷酸被化学封闭,以防止聚合酶在每个循环中掺入一个以上的核苷酸。掺入核苷酸后,在不同通道中针对不同碱基测量荧光信号。关于下一循环,洗涤未掺入的核苷酸,并用TCEP去除3’端的化学封锁。一旦收集到荧光信号,就会开始一个新的循环,重复此动态过程,直到完成每个片段的测序为止。总之,NGS测序反应分三个步骤进行:核苷酸的添加,成像和通过荧光团裂解的3′-OH再生。

 

参考文献

Application of Next Generation Sequencing in Laboratory Medicine.
Authors: Zhong, Yiming and Xu, Feng and Wu, Jinhua and Schubert, Jeffrey and Li, Marilyn M
Journal: Annals of laboratory medicine (2021): 25-43

Current scenario of the genetic testing for rare neurological disorders exploiting next generation sequencing.
Authors: Di Resta, Chiara and Pipitone, Giovanni Battista and Carrera, Paola and Ferrari, Maurizio
Journal: Neural regeneration research (2021): 475-481

A New Type of Chronic Wound Infection after Wisdom Tooth Extraction: A Diagnostic Approach with 16S-rRNA Gene Analysis, Next-Generation Sequencing, and Bioinformatics.
Authors: Böttger, Sebastian and Zechel-Gran, Silke and Streckbein, Philipp and Knitschke, Michael and Hain, Torsten and Weigel, Markus and Wilbrand, Jan-Falco and Domann, Eugen and Howaldt, Hans-Peter and Attia, Sameh
Journal: Pathogens (Basel, Switzerland) (2020)

A novel Next-Generation Sequencing-based approach for concurrent detection of mitochondrial DNA copy number and mutation.
Authors: Zhou, Kaixiang and Mo, Qinqin and Guo, Shanshan and Liu, Yang and Yin, Chun and Ji, Xiaoying and Guo, Xu and Xing, Jinliang
Journal: The Journal of molecular diagnostics : JMD (2020)

Amplicon-Based Next-Generation Sequencing for Detection of Fungi in Formalin-Fixed, Paraffin-Embedded Tissues: Correlation with Histopathology and Clinical Applications.
Authors: Larkin, Paige M K and Lawson, Katy L and Contreras, Deisy A and Le, Catherine Q and Trejo, Marisol and Realegeno, Susan and Hilt, Evann E and Chandrasekaran, Sukantha and Garner, Omai B and Fishbein, Gregory A and Yang, Shangxin
Journal: The Journal of molecular diagnostics : JMD (2020): 1287-1293

Analytical performance evaluation of a commercial next generation sequencing liquid biopsy platform using plasma ctDNA, reference standards, and synthetic serial dilution samples derived from normal plasma.
Authors: Verma, Suman and Moore, Mathew W and Ringler, Rebecca and Ghosal, Abhisek and Horvath, Kyle and Naef, Theodore and Anvari, Sheri and Cotter, Philip D and Gunn, Shelly
Journal: BMC cancer (2020): 945

Author Correction: Ultrasensitive amplicon barcoding for next-generation sequencing facilitating sequence error and amplification-bias correction.
Authors: Ahmed, Ibrahim and Tucci, Felicia A and Aflalo, Aure and Smith, Kenneth G C and Bashford-Rogers, Rachael J M
Journal: Scientific reports (2020): 17010

Automation of Amplicon-Based Library Preparation for Next-Generation Sequencing by Centrifugal Microfluidics.
Authors: Hess, Jacob Friedrich and Kotrová, Michaela and Calabrese, Silvia and Darzentas, Nikos and Hutzenlaub, Tobias and Zengerle, Roland and Brüggemann, Monika and Paust, Nils
Journal: Analytical chemistry (2020): 12833-12841

Characterization of the novel HLA-B*15:474 allele by next-generation sequencing.
Authors: Genebrier, Steve and Elsermans, Vincent and Texeraud, Emeric and Bertrand, Gerald and Renac, Virginie
Journal: HLA (2020)

Correction to: Malignant struma ovarii: next-generation sequencing of six cases revealed Nras, Braf, and Jak3 mutations.
Authors: Poli, Roberta and Scatolini, Maria and Grosso, Enrico and Maletta, Francesca and Gallo, Marco and Liscia, Daniele and Nelva, Anna and Cesario, Flora and Forte, Giuseppe and Metovic, Jasna and Volante, Marco and Arvat, Emanuela and Papotti, Mauro
Journal: Endocrine (2020)

说明书
5-Propargylamino-3′-azidomethyl-dUTP.pdf

1mM TF2-dUTP溶液 货号17007-AAT Bioquest荧光染料

发表于

上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

1mM TF2-dUTP溶液

1mM TF2-dUTP溶液

1mM TF2-dUTP溶液 货号17007 货号 17007 存储条件 在零下15度以下保存, 避免光照
规格 25 nmoles 价格 3924
Ex (nm) 503 Em (nm) 525
分子量 ~1100 溶剂 Water
产品详细介绍

简要概述

产品基本信息

货号:17007

产品名称:1mM TF2-dUTP溶液

规格:25 nmoles

储存条件:-15℃避光防潮

保质期:12个月

 

产品物理化学光谱特性

分子量:~1100

溶剂:水

激发波长(nm):499

发射波长(nm):522

 

产品介绍

1mM TF2-dUTP溶液是美国AAT Bioquest生产的荧光染料,染料修饰的脱氧尿苷5′-三磷酸酯(例如氨基烯丙基-dUTP)可用于通过常规酶促掺入方法(例如逆转录,缺口翻译,随机引物标记或PCR)生产含染料的DNA。这种酶促荧光标记方法广泛用于FISH探针和基于微阵列的实验。该TF2-dUTP共轭物可与Spectrum Green 滤光片组一起用作绿色荧光色。(Spectrum Green 是Vysis的商标)。金畔生物是AAT Bioquest的中国代理商,为您提供最优质的1mM TF2-dUTP溶液。

点击查看光谱

 

参考文献

A visual DNA chip for simultaneous detection of hepatitis B virus, hepatitis C virus and human immunodeficiency virus type-1
Authors: Wen JK, Zhang XE, Cheng Z, Liu H, Zhou YF, Zhang ZP, Yang JH, Deng JY.
Journal: Biosens Bioelectron (2004): 685

Fluorescent DNA hybridization probe preparation using amine modification and reactive dye coupling
Authors: Cox WG, Singer VL.
Journal: Biotechniques (2004): 114

Aminomodified nucleobases: functionalized nucleoside triphosphates applicable for SELEX
Authors: Schoetzau T, Langner J, Moyroud E, Roehl I, Vonhoff S, Klussmann S.
Journal: Bioconjug Chem (2003): 919

Simple method for preparation of fluor/hapten-labeled dUTP
Authors: Nimmakayalu M, Henegariu O, Ward DC, Bray-Ward P.
Journal: Biotechniques (2000): 518

Topology of yeast RNA polymerase II subunits in transcription elongation complexes studied by photoaffinity cross-linking
Authors: Wooddell CI, Burgess RR.
Journal: Biochemistry (2000): 13405

Quantitative analysis of polymerase chain reaction products using biotinylated dUTP incorporation
Authors: Duplaa C, Couffinhal T, Labat L, Moreau C, Lamaziere JM, Bonnet J.
Journal: Anal Biochem (1993): 229

A non-radioisotopic reverse transcriptase assay using biotin-11-deoxyuridinetriphosphate on primer-immobilized microtiter plates
Authors: Urabe T, Sano K, Tanno M, Mizoguchi J, Otani M, Lee MH, Takasaki T, Kusakabe H, Imagawa DT, Nakai M.
Journal: J Virol Methods (1992): 145

Affinity isolation of active murine erythroleukemia cell chromatin: uniform distribution of ubiquitinated histone H2A between active and inactive fractions
Authors: Dawson BA, Herman T, Haas AL, Lough J.
Journal: J Cell Biochem (1991): 166

Non-radioactive labeling and detection of nucleic acids. IV. Synthesis and properties of digoxigenin-modified 2′-deoxyuridine-5′-triphosphates and a photoactivatable analog of digoxigenin (photodigoxigenin)
Authors: Muhlegger K, Huber E, von der Eltz H, Ruger R, Kessler C.
Journal: Biol Chem Hoppe Seyler (1990): 953

说明书
1mM TF2-dUTP溶液.pdf

iFluor 440-dUTP * 1 mM Tris缓冲液(pH 7.5)* 货号17029-AAT Bioquest荧光染料

发表于

上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

iFluor 440-dUTP * 1 mM Tris缓冲液(pH 7.5)*

iFluor 440-dUTP * 1 mM Tris缓冲液(pH 7.5)*

iFluor 440-dUTP * 1 mM Tris缓冲液(pH 7.5)* 货号17029 货号 17029 存储条件 在零下15度以下保存, 避免光照
规格 25 nmoles 价格 1200
Ex (nm) 434 Em (nm) 480
分子量 994.73 溶剂 Water
产品详细介绍

简要概述

产品基本信息

货号:17029

产品名称:iFluor 440-dUTP

规格:25 nmoles

储存条件:-15℃避光防潮

保质期:24个月

 

产品物理化学光谱特性

分子量:994.73

溶剂:水

吸收波长(nm):430

激发波长(nm):434

发射波长(nm):480

消光系数(nm):40000

校正因子(280 nm):0.229

 

产品介绍

染料修饰的脱氧尿苷5′-三磷酸酯(例如氨基烯丙基-dUTP)可用于通过常规酶促掺入方法(例如逆转录,缺口翻译,随机引物标记或PCR)生产含染料的DNA。这种酶促荧光标记方法广泛用于FISH探针和基于微阵列的实验。由于DEAC和SpectrumAqua具有非常相似的光谱特性,DEAC-dUTP缀合物(#17011)与SpectrumAqua 滤波片组(SpectrumAqua 是Vysis的商标)一起使用产生蓝色荧光色。但是,DECA荧光团的极高疏水性使DEAC缀合物易于吸附在塑料表面上,从而导致很高的测定误差。 iFluor 440染​​料具有出色的水溶性,可替代DEAC染料。 iFluor 440-dUTP缀合物是DEAC-dUTP缀合物的优良替代品。 iFluor 440染​​料缀合物比相应的DEAC生物缀合物或其他光谱相似的染料(例如SpectrumAqua)更亮。 iFluor 440荧光团的光谱与SpectrumAqua的滤波片组非常匹配(SpectrumAqua 是Vysis的商标)。

点击查看光谱

 

参考文献

MECOM (EVI1) Rearrangements: A Review and Case Report of Two MDS Patients with Complex 3q Inversion/Deletions.
Authors: Lawce, Helen and Szabo, Elina and Torimaru, Yumi and Davis, Craig and Osterberg, Karin and Olson, Susan and Moore, Steve
Journal: Journal of the Association of Genetic Technologists (2017): 9-14

Localization of a female-specific marker on the chromosomes of the brown seaweed Saccharina japonica using fluorescence in situ hybridization.
Authors: Liu, Yu and Bi, YanHui and Gu, JunGang and Li, LiHua and Zhou, ZhiGang
Journal: PloS one (2012): e48784

Application of tri-colour, dual fusion fluorescence in situ hybridization (FISH) system for the characterization of BCR-ABL1 fusion in chronic myelogenous leukaemia (CML) and residual disease monitoring.
Authors: Siu, Lisa Lp and Ma, Edmond Sk and Wong, Wai Shan and Chan, Man Hong and Wong, Kit Fai
Journal: BMC blood disorders (2009): 4

Review of imaging solutions for integrated quantitative immunohistochemistry in the Pathology daily practice.
Authors: Rojo, Marcial García and Bueno, Gloria and Slodkowska, Janina
Journal: Folia histochemica et cytobiologica (2009): 349-54

Bladder cancer detection using FISH (UroVysion assay).
Authors: Halling, Kevin C and Kipp, Benjamin R
Journal: Advances in anatomic pathology (2008): 279-86

Comparison of quantitative immunofluorescence with conventional methods for HER2/neu testing with respect to response to trastuzumab therapy in metastatic breast cancer.
Authors: Giltnane, Jennifer M and Molinaro, Annette and Cheng, Huan and Robinson, Andrew and Turbin, Dmitry and Gelmon, Karen and Huntsman, David and Rimm, David L
Journal: Archives of pathology & laboratory medicine (2008): 1635-47

AQUA and FISH analysis of HER-2/neu expression and amplification in a small cell lung carcinoma tissue microarray.
Authors: Giltnane, J M and Murren, J R and Rimm, D L and King, B L
Journal: Histopathology (2006): 161-9

A novel tricolor, dual-fusion fluorescence in situ hybridization method to detect BCR/ABL fusion in cells with t(9;22)(q34;q11.2) associated with deletion of DNA on the derivative chromosome 9 in chronic myelocytic leukemia.
Authors: Smoley, Stephanie A and Brockman, Stephanie R and Paternoster, Sarah F and Meyer, Reid G and Dewald, Gordon W
Journal: Cancer genetics and cytogenetics (2004): 1-6

说明书
iFluor 440-dUTP * 1 mM Tris缓冲液(pH 7.5)*.pdf

iFluor 488-dUTP * 1 mM的Tris缓冲液(pH 7.5)* 货号17039-AAT Bioquest荧光染料

发表于

上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

iFluor 488-dUTP * 1 mM的Tris缓冲液(pH 7.5)*

iFluor 488-dUTP * 1 mM的Tris缓冲液(pH 7.5)*

iFluor 488-dUTP * 1 mM的Tris缓冲液(pH 7.5)* 货号17039 货号 17039 存储条件 在零下15度以下保存, 避免光照
规格 25 nmoles 价格 1164
Ex (nm) 491 Em (nm) 516
分子量 1152.83 溶剂 Water
产品详细介绍

简要概述

产品基本信息

货号:17039

产品名称:iFluor 488-dUTP

规格:25 nmoles

储存条件:-15℃避光防潮

保质期:24个月

 

产品物理化学光谱特性

分子量:1152.83

溶剂:水

激发波长(nm):491

发射波长(nm):516

 

产品介绍

染料修饰的脱氧尿苷5′-三磷酸酯是通过常规酶掺入方法(例如反转录,缺口翻译,随机引物标记或PCR)生产染料标记DNA的最常用方法之一。 这种酶促荧光标记方法广泛用于FISH探针和基于微阵列的实验。 该iFluor 488-dUTP缀合物与SpectrumGreen 滤光片组合一起用作绿色荧光(SpectrumGreen 是Vysis的商标)。 与常用的绿色探针(例如Fluorescein-12-dUTP)相比,iFluor 488提供了更明亮的信号,具有很高的光稳定性,并且不受pH值的影响。

点击查看光谱

 

参考文献

Anti-proliferative effect of Fe(III) complexed with 1-(2-hydroxy-3-methoxybenzaldehyde)-4-aminosalicylhydrazone in HepG2 cells.
Authors: Fukushima, Takeshi and Taniguchi, Erina and Yamada, Hiroshi and Kato, Kiyomasa and Shimizu, Ayako and Nishiguchi, Yoshikazu and Onozato, Mayu and Ichiba, Hideaki and Azuma, Yutaro
Journal: Biometals : an international journal on the role of metal ions in biology, biochemistry, and medicine (2015): 669-77

Localisation of abundant and organ-specific genes expressed in Rosa hybrida leaves and flower buds by direct in situ RT-PCR.
Authors: Jedrzejuk, Agata and Mibus, Heiko and Serek, Margrethe
Journal: TheScientificWorldJournal (2012): 609597

SNP genotyping using microsphere-linked PNA and flow cytometric detection.
Authors: Rockenbauer, Eszter and Petersen, Kenneth and Vogel, Ulla and Bolund, Lars and Kølvraa, Steen and Nielsen, Kirsten Vang and Nexø, Bjørn A
Journal: Cytometry. Part A : the journal of the International Society for Analytical Cytology (2005): 80-6

[Comparative genomic hybridization analysis of nasopharyngeal carcinoma drug-resistant cell CNE2/DDP and its parent cell CNE2].
Authors: Jiang, Run-De and Hu, Liang and Guan, Xin-Yuan and Zhang, Li-Xin and Yue, Wen and Cen, Xin-Tang and Li, Chun-Hai
Journal: Ai zheng = Aizheng = Chinese journal of cancer (2004): 386-90

Flow cytometric detection of beta-D-glucuronidase gene in wild-type bacterial cells using in-situ PCR.
Authors: Sachidanandham, Ramaiah and Gin, Karina Yew-Hoong
Journal: Biotechnology and bioengineering (2003): 127-33

Lack of nuclear apoptosis in cardiomyocytes and increased endothelin-1 levels in a rat heart model of myocardial stunning.
Authors: Klainguti, M and Aigner, S and Kilo, J and Eppenberger, H M and Mandinova, A and Aebi, U and Schaub, M C and Shaw, S G and Lüscher, T F and Atar, D
Journal: Basic research in cardiology (2000): 308-15

A method to monitor DNA transfer during transfection.
Authors: Johnson, A L and Jurcisek, J A and Trask, O J and Au, J L
Journal: AAPS pharmSci (1999): E6

Pulsatile shear stress leads to DNA fragmentation in human SH-SY5Y neuroblastoma cell line.
Authors: Triyoso, D H and Good, T A
Journal: The Journal of physiology (1999): 355-65

Detection of TNF alpha and Fas ligand mRNA within synovial mononuclear cells by fluorescence in-cell labeling PCR (FICL-PCR).
Authors: Okubo, M and Brown, M P and Chiba, K and Kasukawa, R and Nishimaki, T
Journal: Molecular biology reports (1998): 217-24

Targeted nucleotide exchange in the alkaline phosphatase gene of HuH-7 cells mediated by a chimeric RNA/DNA oligonucleotide.
Authors: Kren, B T and Cole-Strauss, A and Kmiec, E B and Steer, C J
Journal: Hepatology (Baltimore, Md.) (1997): 1462-8

说明书
iFluor 488-dUTP * 1 mM的Tris缓冲液(pH 7.5)*.pdf

1mM Biotin-16-dUTP溶液 CAS 136632-31-0 货号17017-AAT Bioquest荧光染料

发表于

上海金畔生物科技有限公司代理AAT Bioquest荧光染料全线产品,欢迎访问AAT Bioquest荧光染料官网了解更多信息。

1mM Biotin-16-dUTP溶液 CAS 136632-31-0

1mM Biotin-16-dUTP溶液 CAS 136632-31-0

1mM Biotin-16-dUTP溶液 CAS 136632-31-0 货号17017 货号 17017 存储条件 在零下15度以下保存, 避免光照
规格 25 nmoles 价格 1272
Ex (nm) Em (nm)
分子量 1013.72 溶剂 Water
产品详细介绍

简要概述

产品基本信息

货号:17017

产品名称:1mM 生物素-16-dUTP溶液

CAS:136632-31-0

规格:25nmolse

储存条件:保存在冰箱-15℃干燥

保质期:12个月

 

产品物理化学光谱特性

分子量:1013.72

外观:液体

溶剂:水

激发波长(nm):N/A

发射波长(nm):N/A

 

产品介绍

生物素修饰的脱氧尿苷5′-三磷酸广泛用于各种非放射性DNA标记反应,包括切口平移,随机引物标记,cDNA标记和3’末端标记。已显示生物素化的探针以与非生物素化探针相同的速率和程度与同源核酸杂交。杂交的生物素化DNA探针可以通过抗生物素蛋白和链霉抗生物素蛋白检测。生物素-16-dUTP可以通过切口平移,随机引发,3′-末端标记或在PCR过程中酶促掺入DNA中。数字’16’是dUTP和生物素之间的接头主链中的碳原子数。接头越长,生物素与抗生物素蛋白的相互作用就越有效。另一方面,接头越短,dUTP更有效地掺入DNA。生物素-16-dUTP用于在各种杂交应用中生产生物素化的DNA探针,包括Southern印迹,Northern印迹,斑点印迹,固定细胞和组织。

 

参考文献

A visual DNA chip for simultaneous detection of hepatitis B virus, hepatitis C virus and human immunodeficiency virus type-1
Authors: Wen JK, Zhang XE, Cheng Z, Liu H, Zhou YF, Zhang ZP, Yang JH, Deng JY.
Journal: Biosens Bioelectron (2004): 685

Fluorescent DNA hybridization probe preparation using amine modification and reactive dye coupling
Authors: Cox WG, Singer VL.
Journal: Biotechniques (2004): 114

Aminomodified nucleobases: functionalized nucleoside triphosphates applicable for SELEX
Authors: Schoetzau T, Langner J, Moyroud E, Roehl I, Vonhoff S, Klussmann S.
Journal: Bioconjug Chem (2003): 919

Simple method for preparation of fluor/hapten-labeled dUTP
Authors: Nimmakayalu M, Henegariu O, Ward DC, Bray-Ward P.
Journal: Biotechniques (2000): 518

Topology of yeast RNA polymerase II subunits in transcription elongation complexes studied by photoaffinity cross-linking
Authors: Wooddell CI, Burgess RR.
Journal: Biochemistry (2000): 13405

Quantitative analysis of polymerase chain reaction products using biotinylated dUTP incorporation
Authors: Duplaa C, Couffinhal T, Labat L, Moreau C, Lamaziere JM, Bonnet J.
Journal: Anal Biochem (1993): 229

A non-radioisotopic reverse transcriptase assay using biotin-11-deoxyuridinetriphosphate on primer-immobilized microtiter plates
Authors: Urabe T, Sano K, Tanno M, Mizoguchi J, Otani M, Lee MH, Takasaki T, Kusakabe H, Imagawa DT, Nakai M.
Journal: J Virol Methods (1992): 145

Affinity isolation of active murine erythroleukemia cell chromatin: uniform distribution of ubiquitinated histone H2A between active and inactive fractions
Authors: Dawson BA, Herman T, Haas AL, Lough J.
Journal: J Cell Biochem (1991): 166

Non-radioactive labeling and detection of nucleic acids. IV. Synthesis and properties of digoxigenin-modified 2′-deoxyuridine-5′-triphosphates and a photoactivatable analog of digoxigenin (photodigoxigenin)
Authors: Muhlegger K, Huber E, von der Eltz H, Ruger R, Kessler C.
Journal: Biol Chem Hoppe Seyler (1990): 953

 

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