M-MLV Reverse Transcriptase, RNase H Minus

Catalog No. ON-047
Storage Condition -20℃
Source Recombinant E.coli
Purity >95% by SDS-PAGE

M-MLV Reverse Transcriptase, RNase H Minus

Grade
SKU: ON-047
Unit price:
$0.00

Price

$0.00
Shipping calculated at checkout.
This variant is unavailable. Contact us if you have particular requirements.
Checkout

This variant only support customization. Click the Inquiry button below to submit your custom request to us.

Price/Order Inquiry

Shipping notes

Products in shop.hongene.com currently can only ship to the United States and Canada. For other regions, please visit contact us page to leave us a message or contact our regional sales.

Processing Time: within 2 business days, if available.

Delivery Time:
  • US: 3-8 business days (FedEx Standard).
  • Canada: 5-10 business days (excludes customs delays).

Note: Delays due to force majeure like customs, natural disasters, or strikes are beyond our liability.

Excerpt from Shipping Policy

Details

Product Information

Product description: M-MLV Reverse Transcriptase, RNase H Minus is an RNA-dependent DNA polymerase with no detectable RNase H activity. A point mutation in the RNase H domain increases the thermostablity of the enzyme and support greater cDNA yield of full-length transcripts than wild type M-MLV Reverse Transcriptase.

Source: Recombinant E.coli

Concentration: 200U/μL

Unit Definition: One unit is defined as the amount of enzyme required to catalyze the transfer of 1nmol of deoxynucleotides into acid-precipitable material in 10 minutes at 37℃.

Storage Buffer: 20mM Tris-HCl (pH7.5 at 25℃), 0.1mM EDTA, 200mM NaCl, 0.01% NP-40, 1mM DTT and 50% Glycerol.

Companion Product: 5X RT Reaction Buffer, Cat#ON-067, 250mM Tris-HCl (pH8.3 at 25℃), 375mM KCl, 15mM MgCl2, 50mM DTT.

Key points of operation

  1. Before the first-strand Synthesis of DNA, heat the primer (about 0.5μg) and template (up to 2μg) to 70℃ for 5min to melt secondary structure within the template. Cool the tube on ice to prevent secondary structure from reforming.
  2. Add the following components to the annealed primer/template:
Component
Amount
M-MLW reverse transcriptase, RNase H minus
50-200U
5X RT Reaction Buffer
5μL
RNasin
20U
dNTP (10mM each)
1.25μL
Total
25μL

  1. Incubate for 60min at 42℃.

Security Information

Storage Conditions: -20℃

Quality Assurance: Free of endonuclease, exonuclease, Nickase and RNase activities.

Physical Purity: >95% by SDS-PAGE.

Reference

1. Yu Chen, Weiguo Xu, Qining Sun, Biotechnol Lett. 31, 1051–1057 (2009).

2. Shufeng Liu, Stephen P. Goff, et al. FEBS Letters. 580, 1497-1501(2006).

3. Monica J. Roth, Naoko Tanese, and Stephen P. Goff, The Journal Of Biological Chemistry. 260, 9326-9335(1985).

Specifications
  • Catalog No.
    ON-047
  • Source
    Recombinant E.coli
  • Purity
    >95% by SDS-PAGE
  • Storage Condition
    -20℃

Documentation
COA Contact Us

Product Information

Product description: M-MLV Reverse Transcriptase, RNase H Minus is an RNA-dependent DNA polymerase with no detectable RNase H activity. A point mutation in the RNase H domain increases the thermostablity of the enzyme and support greater cDNA yield of full-length transcripts than wild type M-MLV Reverse Transcriptase.

Source: Recombinant E.coli

Concentration: 200U/μL

Unit Definition: One unit is defined as the amount of enzyme required to catalyze the transfer of 1nmol of deoxynucleotides into acid-precipitable material in 10 minutes at 37℃.

Storage Buffer: 20mM Tris-HCl (pH7.5 at 25℃), 0.1mM EDTA, 200mM NaCl, 0.01% NP-40, 1mM DTT and 50% Glycerol.

Companion Product: 5X RT Reaction Buffer, Cat#ON-067, 250mM Tris-HCl (pH8.3 at 25℃), 375mM KCl, 15mM MgCl2, 50mM DTT.

Key points of operation

  1. Before the first-strand Synthesis of DNA, heat the primer (about 0.5μg) and template (up to 2μg) to 70℃ for 5min to melt secondary structure within the template. Cool the tube on ice to prevent secondary structure from reforming.
  2. Add the following components to the annealed primer/template:
Component
Amount
M-MLW reverse transcriptase, RNase H minus
50-200U
5X RT Reaction Buffer
5μL
RNasin
20U
dNTP (10mM each)
1.25μL
Total
25μL

  1. Incubate for 60min at 42℃.

Security Information

Storage Conditions: -20℃

Quality Assurance: Free of endonuclease, exonuclease, Nickase and RNase activities.

Physical Purity: >95% by SDS-PAGE.

Reference

1. Yu Chen, Weiguo Xu, Qining Sun, Biotechnol Lett. 31, 1051–1057 (2009).

2. Shufeng Liu, Stephen P. Goff, et al. FEBS Letters. 580, 1497-1501(2006).

3. Monica J. Roth, Naoko Tanese, and Stephen P. Goff, The Journal Of Biological Chemistry. 260, 9326-9335(1985).

Related Products

Back to top

My Wishlist