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Restriction Enzymes
    Restriction Enzymes a-b
         Aat II
         Acc I
         Acc II (FnuD II)
         Acc III (BspM II)
         Afa I (Rsa I)
         Afl II
         Alu I
         Aor51H I (Eco47 III)
         Apa I
         ApaL I
         Bal I
         BamH I
         Ban II (HgiJ II)
         Bcn I (Cau II)
         Bgl I
         Bgl II
         Bln I (Avr II)
         BmeT110 I (Ava I)
         Bpu1102 I (Esp I)
         Bsp1286 I (Sdu I)
         Bsp1407 I
         BspT107 I (Hgi C I)
         BssH II (BseP I)
         Bst1107 I (Sna I)
         BstX I
    Restriction Enzymes c-d
    Restriction Enzymes e-f
    Restriction Enzymes g-h
    Restriction Enzymes k-l
    Restriction Enzymes m-n
    Restriction Enzymes o-p
    Restriction Enzymes s-t
    Restriction Enzymes u-v
    Restriction Enzymes w-z


Products >  Molecular_Biology_Tools >  Restriction_Enzymes >  Restriction_Enzymes_a-b >  BlnI

BlnI (AvrII)

DNA restriction enzymes from Takara Bio are unsurpassed in quality and purity. We’ve been producing them for over 30 years and were the first manufacturers to offer commercially available restriction enzymes in Japan. Each lot of every DNA restriction enzyme undergoes stringent quality control tests. Takara Bio DNA restriction enzymes are supplied with optimized buffers that provide maximum activity during restriction enzyme digestion. Visit our Restriction Enzyme Applications pages for information on how to digest DNA, relative activity in each Universal Buffer, star activity, buffers for double digestion, effects of DNA methylation, how to inactivate enzymes, and more.

  At-A-Glance   Documents   Images & Data

Features

DNA Restriction Enzyme: BlnI (AvrII)

C|CTAG G
G GATC|C
  • Source: Brevibacterium linens
  • Concentration: 10 units/ul
  • Supplied buffer: K
  • Reaction temperature: 37°C
  • Substrate for unit definition: lambda DNA
  • Genome DNA analysis: Escherichia coli genome DNA
  • Ligation-recutting test: Ligation efficiency of DNA fragments with cohesive end generated by this enzyme is lower than general 4-base protruding ends. Therefore, more efficient ligation can be achieved by using the reaction conditions for blunt end ligation.
  • Star activity: Cleavage at alternative site(s) occurs in the presence of Mn2+, DMSO, or at high ionic strength.

TaKaRa follows a stringent QC process when manufacturing their restriction enzymes. Each lot of every enzyme undergoes four quality tests including: overdigestion, Genome DNA analysis, Ligation-Recutting and pKF3 Cloning
 
 
Products
Cat. # Product Contents Size Price Units Select
1022A Bln I (Avr II) 400 Units $85.00
1022B Bln I (Avr II) 2,000 Units $335.00
 

 

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