Nucleic acid hybridization

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(Redirected from Nucleic acid hybridisation)

Nucleic acid hybridization is a molecular biology technique that measures the degree of genetic similarity between pools of DNA sequences. It is used to identify the presence of specific sequences in a sample by allowing a labeled nucleic acid probe to form a double-stranded hybrid with complementary sequences in the sample.

Principle[edit | edit source]

The principle of nucleic acid hybridization is based on the ability of complementary nucleic acid strands to form stable double-stranded molecules. When a single-stranded DNA or RNA probe is introduced to a sample containing complementary sequences, the probe will hybridize, or bind, to those sequences. This hybridization can be detected and measured using various methods, such as autoradiography or fluorescence.

Applications[edit | edit source]

Nucleic acid hybridization has a wide range of applications in molecular biology, genetics, and medical diagnostics. Some of the key applications include:

  • Southern blot: Used to detect specific DNA sequences in DNA samples.
  • Northern blot: Used to detect specific RNA sequences in RNA samples.
  • In situ hybridization: Used to detect the location of specific nucleic acid sequences within fixed tissues and cells.
  • Microarray: Used to analyze the expression of thousands of genes simultaneously.
  • Polymerase chain reaction (PCR): Often used in conjunction with hybridization techniques to amplify and detect specific DNA sequences.

Techniques[edit | edit source]

Several techniques are used to perform nucleic acid hybridization, including:

  • **Dot blot hybridization**: A simple method where DNA or RNA samples are spotted onto a membrane and hybridized with a labeled probe.
  • **Colony hybridization**: Used to identify bacterial colonies containing specific DNA sequences.
  • **Filter hybridization**: Involves transferring nucleic acids from a gel to a membrane for hybridization with a probe.

Probes[edit | edit source]

Probes used in nucleic acid hybridization are typically labeled with radioactive isotopes, fluorescent dyes, or enzymes to allow for detection. The choice of label depends on the sensitivity required and the detection method used.

Factors Affecting Hybridization[edit | edit source]

Several factors can influence the efficiency and specificity of nucleic acid hybridization, including:

  • **Temperature**: Higher temperatures can increase the stringency of hybridization, reducing non-specific binding.
  • **Salt concentration**: Higher salt concentrations can stabilize hybridization, while lower concentrations can increase stringency.
  • **Probe length and sequence**: Longer probes and those with higher sequence complementarity to the target will hybridize more efficiently.

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Contributors: Prab R. Tumpati, MD