m1A RNA Enrichment & Quantification Kit
Product Description
N1-methyladenosine (m1A), the methylation of adenosine in the N1 position, is a prevalent and reversible post-transcriptional RNA modification that can occur on messenger RNA (mRNA), transfer RNA (tRNA) and ribosomal RNA (rRNA). Recent studies have revealed the crucial role of m1A RNA modification in multiple cellular processes, including RNA structural stability, folding, interactions with proteins, cell viability, impaired self-renewal ability, cell proliferation, and cell death. Methylated RNA immunoprecipitation (MeRIP) is a popular method to observe and map the location of RNA modifications in specific genes as well as transcriptome-wide.
- Fast, streamlined procedure, finished in 5 hours
- Hands-on time is less than 1 hour
- Enriched RNA for transcriptome-wide profiling
The RayBio® m1A (N1-methyladenosine) RNA Enrichment and quantification kit (QMERIP-M1A) identifies the abundance and enrichment location of m1A by MeRIP and quantitative real-time PCR. The enriched m1A RNA could also be used for transcriptome-wide profiling of m1A. In this assay, RNA sample is digested into fragments consisting of 100~500 nucleotides followed by incubation with an antibody against m1A conjugated to a magnetic bead. Then, the enriched RNA is released, purified, and eluted for qRT-PCR analysis. Included in the kit is a non-immune IgG control conjugated to a magnetic bead and two pairs of primer controls for Hela cell RNA. QMERIP-M1A uses a fast and streamlined procedure so the assay can be finished in 5 hours with a hands-on time of less than 1 hour. This kit has been validated for human, mouse, and rat m1A enrichment.
Workflow
Supporting Data
Figure 2. QMERIP-M1A enrichment test by PCR and RT-qPCR. (A) Representative images of agarose gel running after PCR amplification for the enrichment of m1A targeted APT5A and ACTB mRNA. (B) Bar graph showing the percentage enrichment of m1A targeted APT5A and ACTB mRNA using RT-qPCR assays. 2% Input RNA sample before IP was used as the positive control and IgG-IP was used as the negative control. Almost no PCR products were amplified from the m1A-IP ACTB RNA samples. Error bars, SD (n = 3 independent experiments). *** P-value <0.001 compared to IgG-IP was calculated using the student’s t-test.
