Two-Step RT-qPCR mixes - SYBR Green

Two-Step RT-qPCR mixes - SYBR Green


The two-step RT-qPCR involves two distinct reactions, starting with first strand cDNA synthesis (reverse transcription-RT) and then amplifying part of the resulting cDNA by quantitative PCR in a separate tube . Therefore, two-step RT-qPCR is useful for detecting multiple genes in a single RNA sample. The separation of the RT and quantitative PCR reactions makes it possible to optimize the reaction conditions for each step as well as the flexibility with priming by reverse transcription (oligo (dT) primers, random hexamers or gene-specific primers) and PCR DNA polymerase and PCR components). Compared to one-step RT-qPCR, the disadvantages of two-step RT-qPCR include several steps for extended workflow, additional handling and processing of the sample, and increase the risk of contamination and variation results.

two-step-RT-PCR


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PCR-159S
 192reactions 
PCR-520L
 10x1,25ml 
PCR-520S
 2x1,25ml 
PCR-526L
 10x1,25ml 
PCR-526S
 2x1,25ml 
PCR-532S
 2x1,25ml 
PCR-532L
 10x1,25ml 
PCR-512S
 2x1,25ml 
PCR-512-100ML
 100ml 
PCR-512L
 10x1,25ml 
PCR-523S
 2x1,25ml 
PCR-523L
 10x1,25ml 
PCR-528L
 10x1,25ml 
PCR-528S
 2x1,25ml 
PCR-169S
 192reactions 
PCR-169L
 960reactions 
PCR-159L
 960reactions