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Investigating the Specificity of Restriction Enzymes Simplified Revision Notes

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8.4.3 Investigating the Specificity of Restriction Enzymes

infoNote

Restriction enzymes (restriction endonucleases) are highly specific enzymes used to cut DNA at precise recognition sequences. These enzymes play a crucial role in genetic engineering and recombinant DNA technology.

What Are Restriction Enzymes?

  • Restriction enzymes are proteins originally discovered in bacteria, where they function to protect against viral DNA by cutting it into fragments.
  • Each enzyme recognises a specific DNA sequence (often 4-6 base pairs long) and cuts at or near that site.
  • These sequences are often palindromic, meaning the sequence reads the same forwards and backwards on opposite strands.

Investigating Specificity

  1. Recognition Sequence:
  • Restriction enzymes only cut DNA at their specific recognition site.
  • Example: EcoRI recognises the sequence GAATTC and cuts between G and A.
  1. Sticky Ends vs. Blunt Ends:
  • Enzymes like EcoRI leave sticky ends (single-stranded overhangs), useful for creating recombinant DNA.
  • Others, like SmaI, leave blunt ends (no overhangs), which are less efficient for recombination but still useful for specific applications.
  1. Experimental Methods to Investigate Specificity:
  • DNA is digested with a restriction enzyme and separated using gel electrophoresis to analyse the size of the fragments produced.
  • By using DNA with known sequences, scientists can confirm whether the enzyme cuts only at the expected sites.
  1. Factors Affecting Specificity:
  • Buffer conditions: Specific ions (e.g., magnesium) are required for enzyme activity.
  • Temperature: Most restriction enzymes work optimally at 37°C.
  • Methylation: Methylation of the recognition site can block the enzyme from cutting.

Applications in Genetic Engineering

  • Restriction enzymes are used to:
    • Isolate specific genes from a genome.
    • Prepare DNA fragments for cloning by creating complementary sticky ends.
    • Cut plasmids to insert genes for recombinant DNA production.

Key Terms for Exams

  • Restriction enzyme: Protein that cuts DNA at specific sequences.
  • Recognition sequence: Specific base sequence recognised and cut by the enzyme.
  • Sticky ends: Single-stranded overhangs left after a staggered cut.
  • Blunt ends: Straight cuts with no overhangs.
  • Gel electrophoresis: A technique used to separate DNA fragments by size.
infoNote

Tips:

Ensure you understand the experimental setup for gel electrophoresis and how to interpret the resulting DNA band patterns to identify enzyme specificity.

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