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Safety Information

BLNI-RO

Roche

Bln I (Avr II)

from Brevibacterium linens

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biological source

bacterial (Brevibacterium linens)

Quality Level

100

form

solution

specific activity

10000 U/mL

packaging

pkg of 1,000 U (11558170001 [10 U/μl])
pkg of 200 U (11558161001 [10 U/μl])

manufacturer/tradename

Roche

parameter

37 °C optimum reaction temp.

color

colorless

pH

8.1 (39 °F)

solubility

water: miscible

suitability

suitable for molecular biology

application(s)

life science and biopharma
sample preparation

foreign activity

Endonucleases, none detected (up to 20 U with MWM II-DNA)
Endonucleases, none detected (up to 20U with pBR 322-DNA)

shipped in

dry ice

storage temp.

−20°C

Related Categories

General description

Bln I recognizes the sequence C↓CTAGG and generates fragments with 5′-cohesive termini.

Compatible ends
Bln I ends are compatible with ends generated by Nhe I, Spe I and Xba I.

Isoschizomers
Bln I is an isoschizomer of Avr II.
Note: The complete 13 site Avr II restriction map of the E.coli genome has been reported.

Methylation sensitivity
The enzyme is not known to be affected by methylation.

Specificity

Recognition sites: CCTAGG
CCTAGG
Restriction site: C↓CTAGG
C↓CTAGG
Heat inactivation: No inactivation of Bln I after incubation at 65 °C for 15 minutes.

Quality

Absence of nonspecific endonuclease activities
1 μg λDNA is incubated for 16 hours in 50 μl SuRE/Cut Buffer H with an excess of Bln I. The number of enzyme units which do not change the enzyme-specific pattern is stated in the certificate of analysis.

Absence of exonuclease activity
Approximately 5 μg [3H] labeled calf thymus DNA are incubated with 3 μl Bln I for 4 hours at +37°C in a total volume of 100 μl 50 mM Tris-HCl, 10 mM MgCl2, 1 mM Dithioerythritol, pH approximately 7.5. Under these conditions, no release of radioactivity is detectable, as stated in the certificate of analysis.

Typical ligation and recutting assay
Bln I fragments obtained by complete digestion of 1 μg λ × EcoR I DNA ligated for 16 hours at +4°C with 1 U T4 DNA Ligase in 10 μl buffer that contains 66 mM Tris-HCl, 5 mM MgCl2, 5 mM Dithiothreitol, 1 mM ATP, pH 7.5 (at +20°C). The percentages of product that can be ligated and subsequently recut with Bln I and EcoR I (yielding the typical pattern of λ × EcoR I × Bln I fragments) are stated under "Lig" and "Rec" in the certificate of analysis.

DNA Profile

Number of cleavage sites on different DNAs
  • λ: 2
  • φX174: 0
  • Ad2: 2
  • M13mp7: 0
  • M13mp18:0
  • pBR322: 0
  • pBR328: 0
  • pUC18: 0
  • SV40: 2

Unit Definition

One unit is the enzyme activity that completely cleaves 1 μg λ x EcoR I DNA fragments in one hour at +37 °C in a total volume of 25 μl (1x) SuRE/Cut Buffer H.

Storage and Stability

Do not store below −25°C.

Analysis Note

PFGE tested
Bln I has been tested in Pulsed-Field Gel Electrophoresis (on bacterial chromosomes). For cleavage of genomic DNA (E.coli C 600) embedded in agarose for PFGE analysis, we recommend using 10 U of enzyme/μg DNA and 4 hour incubation.
SuRE/Cut Buffer System
The buffer in bold is recommended for optimal activity
  • A: 25-50%
  • B: 50-75%
  • H: 100%
  • L: 0-10%
  • M: 25-50%

Activity in PCR buffer: Not tested

Other Notes

For life science research only. Not for use in diagnostic procedures.

Kit Components Only

Product No.
Description
  • Enzyme Solution
  • SuRE/Cut Buffer H 10x concentrated

Storage Class Code

12 - Non Combustible Liquids

WGK

WGK 1

Flash Point(F)

does not flash

Flash Point(C)

does not flash

Regulatory Information

常规特殊物品
含少量动物源组分生物产品

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Articles

Restriction Endonucleases - The Molecular Scissors

The term “Restriction enzyme” originated from the studies of Enterobacteria phage λ (lambda phage) in the laboratories of Werner Arber and Matthew Meselson.

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Restriction Enzymes

Restriction endonucleases popularly referred to as restriction enzymes, are ubiquitously present in prokaryotes. The function of restriction endonucleases is mainly protection against foreign genetic material especially against bacteriophage DNA.

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