RevertAid First Strand cDNA Synthesis Kit

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Thermo Scientific™

RevertAid First Strand cDNA Synthesis Kit

Name: RevertAid First Strand cDNA Synthesis Kit
SKU: K1621
Price: 268.00 CNY

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货号	反应次数
K1621	20 次反应
K1622	100 次反应

2 选项

货号 K1621

价格（CNY)

268.00

飞享价

Ends: 31-Dec-2025

446.00

共减 178.00 (40%)

Each

添加至购物车

反应次数:

20 次反应

请求批量或定制报价

价格（CNY)

268.00

飞享价

Ends: 31-Dec-2025

446.00

共减 178.00 (40%)

Each

添加至购物车

Thermo Scientific RevertAid第一链cDNA合成试剂盒包含了足够进行100次x20 μL反应的试剂。本品是以RNA为模板高效合成第一链cDNA的完整系统，可合成长达13kb的cDNA。本品含有RiboLock RNase抑制剂，能够有效保护RNA模板不受降解。
Thermo Scientific RevertAid第一链cDNA合成试剂盒配套提供oligo(dT)18引物和随机六聚体引物。oligo(dT)18引物可以选择性地与mRNA中的poly (A)尾结合。随机六聚体引物无需poly (A)尾，因此可转录mRNA 5’-端区域，也可以无poly (A)尾的RNA (如micoRNA)为模板合成cDNA。该试剂盒也可使用基因特异性引物。

特点：

• 可以高效合成长达13kb的全长第一链cDNA
• 最佳活性温度为42°C
• 完全一提供RT反应所需的所有组分

应用
• 第一链cDNA合成，作为RT-PCR和实时RT-qPCR的模板
• 构建全长cDNA文库
• 反义RNA合成

仅供科研使用。不可用于诊断程序。

规格

最终产品类型第一链 cDNA

产品规格试剂盒

反应次数20 次反应

最佳反应温度42°C

数量20 reactions

反应形式单独组分

试剂类型反转录

逆转录酶RevertAid

核糖核酸酶 H 活性是

运输条件干冰

尺寸（最终产品）长达 13 kb

原始材料RNA

技术反转录

适用于（应用）实时 PCR (qPCR)

反应速度60 min。

Unit SizeEach

内容与储存

• RevertAid 逆转录酶
• RiboLock RNase 抑制剂
• 5X 反应缓冲液
• dNTP 混合物
• Oligo(dT)₁₈ 引物
• 随机六聚体引物
• 对照 GAPDH RNA
• 正向 GAPDH 引物 (10 μM)
• 逆转录 GAPDH 引物 (10 μM)
• 无核酸酶水

储存在 –20°C 下

常见问题解答 (FAQ)

When should I choose regular RevertAid RT or Maxima RT vs. RevertAid H-minus RT or Maxima H-minus RT?

It is generally beneficial to minimize RNase H activity when aiming to produce long transcripts for cDNA cloning. RNase H degrades RNA from RNA-DNA duplexes, which can result in truncated cDNA during reverse transcription of long mRNA. It is also recommended to use RNase H-minus RTs for template-independent addition of C nucleotides. In contrast, reverse transcriptases with intrinsic RNase H activity are often favored in qPCR applications.

Do Thermo Scientific reverse transcriptases (RevertAid RT, RevertAid H-minus RT, Maxima RT, and Maxima H-minus RT) possess terminal deoxynucleotidyl (TdT) activity?

All Thermo Scientific reverse transcriptases possess intrinsic TdT activity although at varying degrees depending upon the reaction conditions. For addition of template-independent C nucleotides (as for SMART and RACE experiments), this specific TdT activity can be induced by Mn2+. We would recommend Maxima H- or RevertAid H- minus RTs for this purpose.

What steps should I take while performing first strand cDNA synthesis using low purity template (e.g., inhibitors in RNA sample)?

Trace amounts of reagents used in RNA purification protocols may remain in solution and inhibit first-strand synthesis, e.g., SDS, EDTA, guanidine salts, phosphate, pyrophosphate, polyamines, spermidine. To remove trace contaminants, we recommend re-precipitating the RNA with ethanol and washing the pellet with 75% ethanol, or re-purifying the RNA.

For reverse transcription, how important is the quality of RNA template?

RNA purity and integrity are essential for synthesis and quantification of cDNA. Always assess the integrity of RNA prior to cDNA synthesis. Use freshly prepared RNA. Multiple freeze/thaw cycles of the RNA sample and synthesized cDNA is not recommended. Avoid RNase contamination and discard low quality RNA.

When should I choose regular RevertAid RT or Maxima RT vs. RevertAid H Minus RT or Maxima H Minus RT?

It is generally beneficial to minimize RNase H activity when aiming to produce long transcripts for cDNA cloning. RNase H degrades RNA from RNA-DNA duplexes, which can result in truncated cDNA during reverse transcription of long mRNA. It is also recommended to use RNase H Minus RTs for template-independent addition of C nucleotides. In contrast, reverse transcriptases with intrinsic RNase H activity are often favored in qPCR applications.

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