DNA-probe - ορισμός. Τι είναι το DNA-probe
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Τι (ποιος) είναι DNA-probe - ορισμός

A PIECE OF DNA OR RNA THAT IS RADIOACTIVELY OR FLUORESCENTLY LABELED FOR DIAGNOSTIC TESTS.
DNA probe; Gene probe; Probe hybridization; Dna probes; Rna probes; Dna probe; DNA probes; RNA probe; Radioactive probes

Test probe         
  • High voltage resistor divider probe for voltages up to 50 kV. The probe tip consists of a ''corona ball'', which avoids corona discharge and arcing by distributing the electric field gradient.
  • A pair of simple test leads
  • A passive oscilloscope probe with a switch in the probe handle that selects 1× or 10× attenuation
  • A thermocouple probe
  • A tweezer probe
PROBE USED FOR ELECTRONIC TESTING
Test prod; Scope probe; Oscilloscope probe; Test lead; Differential probe; Near-field probe; Near field probe; Z0 probe; Zo probe; ZO probe; High voltage probe
A test probe is a physical device used to connect electronic test equipment to a device under test (DUT). Test probes range from very simple, robust devices to complex probes that are sophisticated, expensive, and fragile.
Hybridization probe         
In molecular biology, a hybridization probe (HP) is a fragment of DNA or RNA of usually 15–10000 nucleotide long which can be radioactively or fluorescently labeled. HP can be used to detect the presence of nucleotide sequences in analyzed RNA or DNA that are complementary to the sequence in the probe.
DNA glycosylase         
  • 
Hydrolysis of cytosine to uracil
ENZYMES INVOLVED IN BASE EXCISION REPAIR
GO system; Dna glycosylases; Dna glycosylase; DNA glycosylases; Dna Glycosylase
DNA glycosylases are a family of enzymes involved in base excision repair, classified under EC number EC 3.2.

Βικιπαίδεια

Hybridization probe

In molecular biology, a hybridization probe (HP) is a fragment of DNA or RNA of usually 15–10000 nucleotide long which can be radioactively or fluorescently labeled. HP can be used to detect the presence of nucleotide sequences in analyzed RNA or DNA that are complementary to the sequence in the probe. The labeled probe is first denatured (by heating or under alkaline conditions such as exposure to sodium hydroxide) into single stranded DNA (ssDNA) and then hybridized to the target ssDNA (Southern blotting) or RNA (northern blotting) immobilized on a membrane or in situ.

To detect hybridization of the probe to its target sequence, the probe is tagged (or "labeled") with a molecular marker of either radioactive or (more recently) fluorescent molecules. Commonly used markers are 32P (a radioactive isotope of phosphorus incorporated into the phosphodiester bond in the probe DNA), digoxigenin, a non-radioactive, antibody-based marker, biotin or fluorescein. DNA sequences or RNA transcripts that have moderate to high sequence similarity to the probe are then detected by visualizing the hybridized probe via autoradiography or other imaging techniques. Normally, either X-ray pictures are taken of the filter, or the filter is placed under UV light. Detection of sequences with moderate or high similarity depends on how stringent the hybridization conditions were applied—high stringency, such as high hybridization temperature and low salt in hybridization buffers, permits only hybridization between nucleic acid sequences that are highly similar, whereas low stringency, such as lower temperature and high salt, allows hybridization when the sequences are less similar.

Hybridization probes used in DNA microarrays refer to DNA covalently attached to an inert surface, such as coated glass slides or gene chips, to which a mobile cDNA target is hybridized. Depending on the method, the probe may be synthesized using the phosphoramidite method, or it can be generated and labeled by PCR amplification or cloning (both are older methods). In order to increase the in vivo stability of the probe RNA is not used. Instead, RNA analogues may be used, in particular morpholino- derivatives. Molecular DNA- or RNA-based probes are routinely used in screening gene libraries, detecting nucleotide sequences with blotting methods, and in other gene technologies, such as nucleic acid and tissue microarrays.