4-RNA Methylation Dot Blot Combination Kit

This is a combined m1A, m7G, m6A, and m5C dot blot assay kit for quantifying the 4 most common global RNA modification levels in RNA, urine, serum, plasma, or other nucleic samples.
$900.00
In stock
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Product Description

Specifications

Size 1 Kit
Species Human, Mouse, Rat
Quantitative/Semi-Quantitative Semi-Quantitative
Compatible Sample Types Plasma, Serum, Extracted RNA
Research Area Methylation, Epigenetics
Estimated Lead Time 1-2 business days
Shipping Type Blue ice
Storage 4°C
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Introduction

RNA modifications are dynamic and reversible chemical modifications on substrate RNA that are regulated by specific modifying enzymes. They play important roles in the regulation of many biological processes in various diseases, including cancer, neurological disorders, cardiovascular diseases, metabolic diseases, genetic and developmental diseases, as well as immune disorders.

Advanced sequencing technologies have increasingly highlighted the significance of RNA modifications in human diseases which caught increasing attention in scientific research. Recent studies have mapped out the locations and abundance of key RNA modifications, such as N6-methyladenosine (m6A), 5-methylcytosine (m5C), N1-methyladenosine (m1A), and N7-methylguanosine (m7G), primarily through antibody immunoprecipitation or chemical treatments coupled with next-generation sequencing. It is well known that through the “writing (Methyltransferase) - erasing (Demethyltransferase) -reading (Binding protein)” mechanisms, RNA modifications regulate the stability, translation, and localization of pivotal disease-related mRNAs to manipulate disease development. Further research into RNA modifications, their roles, inhibitors, and activators, is essential for disease diagnosis, treatment, and prognosis.

Here, we introduce a combined m1A, m7G, m6A, and m5C dot blot kit, which offers a reliable, simple, and rapid method of quantifying the 4 most common global RNA modification levels in RNA, urine, serum, plasma, or other nucleic samples collected from humans, rats, and mice.

Product Features

  • Highly sensitive and specific
  • Requires minimal sample preparation
  • No specialty equipment required
  • Convenient for high-throughput screening in large-scale studies
  • ≥ 48 samples could be detected by 1 kit

Kit Components

Component Size / Description
m1A Antibody 1 vial
m7G Antibody 1 vial
m6A Antibody 1 vial
m5C Antibody 1 vial
Anti-Rabbit IgG-HRP Antibody 1 vial
Detection Buffer C 1 bottle
Detection Buffer D 1 bottle
Wash Buffer 1 1 bottle
Blocking Buffer 1 bottle
Methylene Blue Staining Buffer 1 bottle
NC Membranes 4 sheets
Plastic Sheet 8 sheets
Incubation Dish 1 box

Additional Materials Required

  • RNase-free tubes
  • Heat blocker
  • 10 cm plastic petri dish
  • UV cross-linker
  • Chemiluminescent Imaging system

Assay Procedure Summary

  1. Sample preparation: Depending on the type of sample (RNA, plasma, or serum), different methods of extraction, dilution, and denaturation are required.
  2. Sample loading and crosslinking: The sample is spotted onto a nitrocellulose membrane, air dried, and crosslinked with UV light twice.
  3. Methylene blue staining: One line of the spotted sample replicates is cut off and stained with methylene blue buffer to serve as an internal control.
  4. Blocking and antibody incubation: The membrane is blocked with blocking buffer and then incubated with anti-m1A antibody and HRP-conjugated secondary antibody.
  5. Detection and imaging: The membrane is treated with a mixture of detection buffers C and D, which catalyzes a color development reaction. The chemiluminescent signal is captured by an imaging system.

Typical Data

Typical Data      Typical Data

Storage/Stability

The entire kit may be stored at -20°C to -80°C for up to 12 months from the date of shipment. For extended storage, it is recommended to store it at -80°C. Avoid repeated freeze-thaw cycles.

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