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관련 카테고리
일반 설명
Rapid Amplification of cDNA ends (RACE) is a prevalent technique used to rapidly obtain full-length cDNA from partially known sequences.[1] The 5′/3′ RACE kit contains Transcriptor Reverse Transcriptase and recombinant Terminal Transferase. Transcriptor Reverse Transcriptase transcribes full-length cDNA for the highly sensitive and rapid amplification of either 5′ or 3′ cDNA fragments up to 14 kb. Due to its thermostability (up to +65 °C), it can work with GC-rich templates with high secondary structure. High sensitivity can be achieved using Transcriptor Reverse Transcriptase, resulting in highly efficient cDNA synthesis and the generation of long RACE products. Recombinant Terminal transferase is used to add a homopolymeric A-tail to the 3′ end of the cDNA.[2] The poly(A)+ tail decreases the likelihood of inappropriate truncation by the oligo(dT)-anchor primer, and overcomes the weaker A/T compared to the G/C hybridization. Moreover, longer stretches of A residues are required before the oligo(dT)-anchor primer can hybridize to an internal site and can truncate the amplification product. Tailed cDNA is amplified by PCR using a gene-specific primer and the oligo(dT)-anchor primer. The obtained cDNA is further amplified by a second PCR using a nested specific primer and the PCR-anchor primer, allowing RACE products to be cloned into an appropriate vector for subsequent studies.
특이성
Heat inactivation: Terminal Transferase: 70 °C for 10 minutes
Transcriptor Reverse Transcriptase: 85 °C for 5 minutes
Transcriptor Reverse Transcriptase: 85 °C for 5 minutes
애플리케이션
5′/3′ RACE Kit, 2nd Generation is suitable for
- Structural and expression studies of RNA molecules[3]
- Generating full-length cDNAs[4][5]
- Isolation and characterization of 5′ or 3′ ends from low-copy RNA messages[6]
- first strand cDNA synthesis[6]
- Amplification and further cloning of rare mRNAs[6]
- Use in conjunction with exon-trapping methods
- Products of the RACE reaction can be directly sequenced without cloning
특징 및 장점
- Robust performance: Recombinant Transcriptor Reverse Transcriptase allows procession through regions of difficult secondary RNA structure.
- Convenient: Function and expression studies of either 5′ or 3′ end of the RNA can be performed with the same kit.
- Reliable: dA tailing of cDNA with Recombinant Terminal Transferase decreases the likelihood of inappropriate truncation.
- Reproducible: Oligo dT-anchor primer with non 3′dT ensures correct binding to the inner end of the poly (A) tail.
- Produce long fragments: Generate cDNA up to 14kb in length with Transcriptor Reverse Transcriptase.
The control reaction includes transcription of the control RNA into first-strand cDNA using the control primer neo1/rev. Amplification of the cDNA is performed using the control primer neo2/rev and neo3/for to obtain a 157-bp PCR product. Tailing of the purified cDNA is performed with dATP. Amplification of the tailed cDNA is performed with oligo dT-anchor primer and the control primer neo2/rev to obtain a 293-bp PCR product.
포장
1 kit containing 12 components
기타 정보
For life science research only. Not for use in diagnostic procedures.
키트 구성품 전용
제품 번호
설명
- cDNA Synthesis Buffer 5x concentrated
- Transcriptor Reverse Transcriptase 20 U/μl
- Deoxynucleotide Mix
- dATP, pH 7.5 (20 °C)
- Reaction Buffer 10x concentrated
- Terminal Transferase, recombinant
- Control neo-RNA 1 ng/μl
- Oligo dT-Anchor Primer
- PCR Anchor Primer
- Control Primer neo1/rev primer 12.5 μM
- Control Primer neo2/rev primer 12.5 μM
- Control Primer neo3/for primer 12.5 μM
모두 보기 (12)
Storage Class Code
12 - Non Combustible Liquids
WGK
WGK 1
Flash Point (°F)
does not flash
Flash Point (°C)
does not flash
이미 열람한 고객
Dilek Cansu Gurer et al.
Frontiers in cell and developmental biology, 9, 688855-688855 (2021-09-10)
Cisplatin is a well-known cancer chemotherapeutic agent but how extensively long non-coding RNA (lncRNA) expression is modulated by cisplatin is unknown. It is imperative to employ a comprehensive approach to obtain a better account of cisplatin-mediated changes in the expression
Rapid amplification of 5 [prime] complementary DNA ends (5 [prime] RACE)
Sambrook J and Russell DW
Nature methods, 2, 629-630 (2005)
Erdong Cheng et al.
Journal of virology, 86(18), 10173-10185 (2012-07-13)
Hantaviruses, similarly to other negative-strand segmented RNA viruses, initiate the synthesis of translation-competent capped mRNAs by a unique cap-snatching mechanism. Hantavirus nucleocapsid protein (N) binds to host mRNA caps and requires four nucleotides adjacent to the 5' cap for high-affinity
D Chen et al.
BioTechniques, 30(3), 574-580 (2001-03-17)
In determining the terminal sequences of the genomic dsRNAs of rotavirus by 5'-rapid amplification of cDNA ends (5'-RACE), it was found that most of the viral cDNAs contained extra nucleotides at their 5' termini that had not been reported before
Ramesh Choudhari et al.
Molecular and cellular endocrinology, 510, 110819-110819 (2020-04-21)
Recent technical and other advances in genomics provide unique opportunities to improve our understanding of human physiology and disease predisposition through a detailed analysis of gene structure and expression by examining data in public genome and gene-expression repositories. Yet, the
문서
In addition to the troubleshooting provided in the product manual, most probably the efficiency of the tailing reaction performed by Terminal Transferase could be impaired. This could occur due to several reasons (which will not only affect the control reaction, but 5′ RACE in general):
자사의 과학자팀은 생명 과학, 재료 과학, 화학 합성, 크로마토그래피, 분석 및 기타 많은 영역을 포함한 모든 과학 분야에 경험이 있습니다..
고객지원팀으로 연락바랍니다.
