Fluorescence In Situ Hybridization (FISH) is a molecular cytogenetic technique that enables the detection and localization of specific nucleic acid sequences within fixed cells, chromosomes, or tissue sections using fluorescently labeled probes. The probe is the core reagent in FISH, as its design, composition, labeling, and hybridization properties fundamentally determine the assay's specificity, sensitivity, and resolution.
Nature and Types of FISH Probes
FISH probes are nucleic acid sequences—commonly DNA, cDNA, or RNA—that are designed to be complementary to the target sequence of interest. They may be:
- Single-stranded or double-stranded nucleic acids
- Of varying length: from short oligonucleotides (~20–50 bases) to large DNA fragments (hundreds to thousands of bases)
- Derived either from cloned DNA (plasmids, cosmids, PACs, YACs, BACs) or synthetically prepared oligonucleotides
Probes can target unique gene regions, chromosomal loci, or entire chromosomes (whole-chromosome paints used in metaphase spreads) depending on the experimental goals.
Sources and Preparation
Cloned DNA Probes: DNA fragments harboring the sequence of interest are isolated from vectors such as plasmids or bacterial artificial chromosomes. These fragments allow targeting specific genes or genomic regions.
Synthetic Oligonucleotide Probes: Short, chemically synthesized sequences allow high specificity and rapid synthesis for known target sequences.
Ribosomal RNA (rRNA) Probes: Used extensively in microbial ecology for detecting bacterial groups by targeting 16S or 23S rRNA.
Labeling Strategies
For detection, probes must carry a fluorescent label either directly or indirectly:
Direct Labeling: Fluorochrome-modified nucleotides (e.g., Cy3, FITC) are incorporated during probe synthesis (nick translation, random priming, or PCR-based methods). This approach permits immediate visualization after hybridization.
Indirect Labeling: Probes are labeled with hapten-conjugated nucleotides (e.g., biotin-11-dUTP, digoxigenin). Post-hybridization, fluorescently tagged antibodies or streptavidin bind to the hapten, amplifying signals and allowing multiplex detection with different reporters.
Hybridization Conditions
Probes must be denatured to single strands to hybridize with the complementary target DNA or RNA, usually by heat treatment in the presence of denaturation buffers (often containing 50% formamide). The hybridization step is then conducted at optimized temperatures (37–42 °C), aided by hybridization buffers that enhance binding kinetics and specificity.
Probe Specificity and Validation
The specificity of a probe depends on its sequence and the stringency of hybridization conditions (salt concentration, temperature, and formamide content). Validation of probes involves testing against target and non-target sequences:
- Carefully optimized formamide concentrations enable discrimination of sequences differing by as little as one or two nucleotides.
- Experimental validation includes hybridization to known positive and negative control samples.
Applications of FISH Probes
- Identification of chromosome abnormalities in clinical diagnostics (e.g., detecting translocations, deletions)
- Detection of pathogens or bacterial taxa in environmental or medical samples via rRNA-targeted probes
- Gene mapping and characterization in research settings
- Microbial community profiling using fluorescent oligonucleotide probes targeting conserved regions of rRNA
Summary
The nature and quality of the probes strongly determine FISH performance. Probes typically consist of fluorescently labeled DNA or RNA sequences complementary to the target nucleic acid, prepared by cloning or synthesis, and labeled directly or indirectly for fluorescence detection. Their successful application relies on precise design, effective labeling, and optimized hybridization conditions to achieve sensitive and specific detection within the complex environment of cells or tissues.