RNase A (10 mg/mL)

SKU:BHZ20800059 Enzymes & Molecular Biology
Overview
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Ribonuclease A (RNase A) is a single-stranded polypeptide containing 4 disulfide bonds with a molecular weight of about 13.7 kDa. RNase A is an endoribonuclease that specifically degrades single-stranded RNA at C and U residues. Specifically, the cleavage recognizes the phosphodiester bond formed by
Enzyme Type Nucleases
Grade RUO
Storage -20°C
Shipping Dry Ice
Options selector
Catalog no. Size
10405ES03 1 mL
10405ES10 10 mL
Available Options

Select the variant that best fits your experiment. Availability and lead time may vary by option.

  • Options:
    • Size (2) - 1 mL, 10 mL
  • Lead time: options listed in "Availability Content"; otherwise, there will be a column of "lead time", other statuses may take longer.
  • Storage: -20°C
  • Shipping: cold-chain shipment (typically with ice packs).
  • Upon receipt: store at the recommended temperature as soon as possible.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No 10405ES
Product Type
  • Enzymes
  • Nucleases
Shipping Dry Ice
Source Recombinant (E. coli)
Storage -20°C

Ribonuclease A (RNase A) is a single-stranded polypeptide containing 4 disulfide bonds with a molecular weight of about 13.7 kDa. RNase A is an endoribonuclease that specifically degrades single-stranded RNA at C and U residues. Specifically, the cleavage recognizes the phosphodiester bond formed by the 5'-ribose of a nucleotide and the phosphate group on the 3'-ribose of the adjacent pyrimidine nucleotide, so that the 2', 3' - Cyclic phosphates are hydrolyzed to the corresponding 3'-nucleoside phosphates (eg, pG-pG-pC-pA-pG is cleaved by RNase A to generate pG-pG-pCp and A-PG).RNase A is the most active in cleaving single-stranded RNA .Recommended working concentration is 1-100 μ G/mL, compatible with various reaction systems. Low salt concentration (0-100 mM NaCl) can be used to cut single-stranded RNA, double-stranded RNA, and RNA chains formed by RNA-DNA hybridization. However, at high salt concentration (≥ 0.3 M), RNase A only specifically cleaves single-stranded RNA.

RNase A is most commonly used to remove RNA during the preparation of plasmid DNA or genomic DNA. Whether or not DNase is active during the preparation process can easily affect the reaction. The traditional method of boiling in a water bath can be used to inactivate DNase activity. This product does not contain DNase and protease, and does not require heat treatment before use. In addition, this product can also be used in molecular biology experiments such as RNase protection analysis and RNA sequence analysis.

This product is provided as a solution at a concentration of 100 mg/mL. The recommended working concentration is 1-100 μg/mL, depending on the type of application.

Features

  • Ribonuclease A (RNase A), from bovine pancreas
  • Activity ≥80 Kunitz U/mg
  • No DNase residue

Applications

  • RNases
  • Epitranscriptome Analysis
  • Genomic DNA Extraction & Purification

Specifications

Components No.

Name

10406ES03

10405ES03

RNase A (10 mg/mL)

1 mL

 10405ES10

RNase A (10 mg/mL)

10 mL 

Glycerol Content

Contains Glycerol

Shipping and Storage

The product should be stored at -25°C ~ -15℃ for 1 years.

The preservation buffer was 50 mM Tris-HCl (pH 7.4) and 50% (V/V) glycerol.

Store this enzyme at -20°C and avoid repeated freeze-thaw cycles to preserve catalytic activity. The product is shipped Dry Ice and remains stable for up to one year from the date of manufacture when stored under recommended conditions. Aliquoting the stock solution into single-use volumes is recommended for enzymes used infrequently to minimize thermal cycling of the bulk stock.

RNases Epitranscriptome Analysis Genomic DNA Extraction & Purification. Always verify compatibility with your specific template, buffer, and downstream workflow.

One unit (U) is defined as the amount of enzyme that degrades 1 µg of DNA or RNA substrate to acid-soluble form in 30 min at 37°C under defined buffer conditions.

This enzyme is produced as Recombinant (E. coli) and supplied as a Research Use Only (RUO) reagent. Each lot is subjected to activity assay, purity assessment by SDS-PAGE, and functional validation prior to release. A Certificate of Analysis (CoA) and Safety Data Sheet (SDS) are available on request.

Nuclease activity typically requires divalent metal ion cofactors (Mg²⁺ or Mn²⁺ at 1–5 mM). Activity is inhibited by chelating agents such as EDTA (≥1 mM), high salt concentrations, and reducing agents such as DTT at elevated concentrations. Heat inactivation (65–75°C for 15 min) is effective for most nucleases, allowing removal of enzyme activity after digestion without column purification.

Yeasen Biotechnology supports custom enzyme solutions across multiple service lines — from GMP-grade bulk supply to directed enzyme engineering. Contact BioHippo to discuss requirements and initiate a project inquiry.

▶ GMP-Grade & Bulk Supply

Select Yeasen enzymes are available in GMP grade, manufactured in an ISO 13485-certified UCF.ME™ ultra-clean molecular enzyme facility with FDA Drug Master File (DMF) support.

  • GMP-grade release testing and CoA documentation
  • ISO 13485-certified production facility
  • Scalable from milligram to multi-gram quantities
  • Consistent lot-to-lot activity specifications

▶ Glycerol-Free & Custom Formulation

Glycerol-free enzyme formats are available for applications requiring lyophilization compatibility, liquid handling automation, or direct IVD master mix integration.

  • Glycerol-free liquid format (standard and custom buffers)
  • Lyophilization-ready enzyme preparation
  • Custom reaction buffer optimization for specific assay conditions
  • Compatible with freeze-drying workflows for point-of-care formats

▶ Molecular IVD RDC Service

Yeasen's Research and Development Contracting (RDC) team delivers end-to-end solutions for molecular diagnostic product development, covering enzyme selection through clinical validation support.

  • Enzyme selection and performance matching
  • Primer/probe design and reaction buffer optimization
  • Sensitivity, specificity, and precision validation studies
  • Stability studies and SNP evaluation
  • Instrument platform compatibility assessment

▶ ZymeEditor™ Enzyme Engineering

Yeasen's proprietary ZymeEditor™ directed evolution and rational design platform enables the development of custom enzyme variants with tailored performance characteristics not available in off-the-shelf products.

  • Directed evolution for enhanced thermostability, processivity, or fidelity
  • Rational design for altered substrate specificity or cofactor requirements
  • Library screening from Yeasen's proprietary enzyme variant collection
  • Scale-up to commercial quantities upon candidate confirmation

ⓘ Customization services are fulfilled by Yeasen Biotechnology. Lead times and minimum order quantities vary by service type. Contact BioHippo for project scoping and pricing.

  1. Chen Q, Xin M, Wang L, et al. Inhibition of LDHA to induce eEF2 release enhances thrombocytopoiesis. Blood. 2022;139(19):2958-2971. doi:10.1182/blood.2022015620(IF:23.629)
  2. Chen K, Guo T, Li XM, et al. Translational Regulation of Plant Response to High Temperature by a Dual-Function tRNAHis Guanylyltransferase in Rice. Mol Plant. 2019;12(8):1123-1142. doi:10.1016/j.molp.2019.04.012(IF:10.812)

What is the magic of RNase A? Uncovering its diverse applications

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Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

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Try Celltrypse Free – Request Your Sample Today

Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

Try Celltrypse Free – Request Your Sample Today