DNase I (RNase-free)

Catalog No. ON-109
Purity >95% by SDS-PAGE
Storage Condition -20℃
Source Recombinant E.coli

DNase I (RNase-free)

Grade
GMP level
Amount/Package: 1kU / centrifuge tube
SKU: ON-109-KU001-P
Unit price:
$25.00

Price

$25.00
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Details

Product Information

DNase I (RNase free) is an endonuclease that digests single- and double-stranded DNA. It nonspecifically cleaves DNA to release di-,tri- and oligonucleotide products with 5'-phosphorylated and 3'-hydroxylated end.

Source: Recombinant E.coli
Concentration: 1U/μL
Unit Definition: One unit is defined as the amount of enzyme required to completely degrade 1μg of λDNA in 10 minutes at 37℃.
Storage Buffer: 50mM Tris-HCl (pH7.5, 25℃), 10mM CaCl2 and 50% Glyercol

Companion Product:


Key points of operation

DNase I treatment after IVT reaction:

  1. Directly add DNase I (1unit DNase I per ug of DNA template) to IVT Reaction, mix well and incubate 30 min at 37°C.
  2. Add 0.5M EDTA to a final concertation over one millimole than divalent cations.
  3. Heat inactivate at 75℃ for 10min.

Security Information

Storage Conditions: -20℃
Quality Assurance: Free of RNase activities.
Physical Purity: >95% by SDS-PAGE.


Reference

1. A F Worrall,B A Connolly, J,Biol,Chem. 265,21889–21896 (1990).
2. Ching-Ying Chen,Shao-Chun Lu,et al. Gene. 206, 181-184(1998).

Specifications

  • Catalog No.
    ON-109
  • Source
    Recombinant E.coli
  • Purity
    >95% by SDS-PAGE
  • Storage Condition
    -20℃

Documentation

Product Information

DNase I (RNase free) is an endonuclease that digests single- and double-stranded DNA. It nonspecifically cleaves DNA to release di-,tri- and oligonucleotide products with 5'-phosphorylated and 3'-hydroxylated end.

Source: Recombinant E.coli
Concentration: 1U/μL
Unit Definition: One unit is defined as the amount of enzyme required to completely degrade 1μg of λDNA in 10 minutes at 37℃.
Storage Buffer: 50mM Tris-HCl (pH7.5, 25℃), 10mM CaCl2 and 50% Glyercol

Companion Product:


Key points of operation

DNase I treatment after IVT reaction:

  1. Directly add DNase I (1unit DNase I per ug of DNA template) to IVT Reaction, mix well and incubate 30 min at 37°C.
  2. Add 0.5M EDTA to a final concertation over one millimole than divalent cations.
  3. Heat inactivate at 75℃ for 10min.

Security Information

Storage Conditions: -20℃
Quality Assurance: Free of RNase activities.
Physical Purity: >95% by SDS-PAGE.


Reference

1. A F Worrall,B A Connolly, J,Biol,Chem. 265,21889–21896 (1990).
2. Ching-Ying Chen,Shao-Chun Lu,et al. Gene. 206, 181-184(1998).

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With nearly 30 years of expertise, we control a secure supply chain for RNA raw materials and provide reliable GMP-grade oligo synthesis from research to commercial kilogram-scale production.

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We implement multiple stringent QC steps, maintain ISO certifications, and ensure >99% batch-to-batch consistency, reducing scale-up and PPQ risks.

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Hongene operates a 1.67-million-square-foot oligonucleotide manufacturing facility featuring advanced equipment, including multiple OligoPilot™ and OligoProcess™ synthesizers ranging from 10 to 1,800 mmol. Its 48 flexible production lines enable seamless, one-stop scale-up of API production from gram-level quantities to metric tons, achieving purity of ≥98% while supporting compliance with NMPA, FDA, and EMA regulatory requirements.

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