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Wikipedia

Fluorescence in situ hybridization

January 01, 1970

Fluorescence in situ hybridization (FISH) is a molecular cytogenetic technique that uses fluorescent probes that bind to only particular parts of a nucleic acid sequence with a high degree of sequence complementarity. It was developed by biomedical researchers in the early 1980s[1] to detect and localize the presence or absence of specific DNA sequences on chromosomes. Fluorescence microscopy can be used to find out where the fluorescent probe is bound to the chromosomes. FISH is often used for finding specific features in DNA for use in genetic counseling, medicine, and species identification.[2] FISH can also be used to detect and localize specific RNA targets (mRNA, lncRNA and miRNA)[citation needed] in cells, circulating tumor cells, and tissue samples. In this context, it can help define the spatial-temporal patterns of gene expression within cells and tissues.

Multiplex RNA visualization in cells using ViewRNA FISH Assays
A metaphase cell positive for the bcr/abl rearrangement (associated with chronic myelogenous leukemia) using FISH. The chromosomes can be seen in blue. The chromosome that is labeled with green and red spots (upper left) is the one where the rearrangement is present.

Probes – RNA and DNA edit

 
ViewRNA detection of miR-133(green) and myogenin mRNA (red) in C2C12 differentiating cells

In biology, a probe is a single strand of DNA or RNA that is complementary to a nucleotide sequence of interest.

RNA probes can be designed for any gene or any sequence within a gene for visualization of mRNA,[3][4][5] lncRNA[6][7][8] and miRNA in tissues and cells. FISH is used by examining the cellular reproduction cycle, specifically interphase of the nuclei for any chromosomal abnormalities.[9] FISH allows the analysis of a large series of archival cases much easier to identify the pinpointed chromosome by creating a probe with an artificial chromosomal foundation that will attract similar chromosomes.[9] The hybridization signals for each probe when a nucleic abnormality is detected.[9] Each probe for the detection of mRNA and lncRNA is composed of ~20-50 oligonucleotide pairs, each pair covering a space of 40–50 bp. The specifics depend on the specific FISH technique used. For miRNA detection, the probes use proprietary chemistry for specific detection of miRNA and cover the entire miRNA sequence.

 
Urothelial cells marked with four different probes

Probes are often derived from fragments of DNA that were isolated, purified, and amplified for use in the Human Genome Project. The size of the human genome is so large, compared to the length that could be sequenced directly, that it was necessary to divide the genome into fragments. (In the eventual analysis, these fragments were put into order by digesting a copy of each fragment into still smaller fragments using sequence-specific endonucleases, measuring the size of each small fragment using size-exclusion chromatography, and using that information to determine where the large fragments overlapped one another.) To preserve the fragments with their individual DNA sequences, the fragments were added into a system of continually replicating bacteria populations. Clonal populations of bacteria, each population maintaining a single artificial chromosome, are stored in various laboratories around the world. The artificial chromosomes (BAC) can be grown, extracted, and labeled, in any lab containing a library. Genomic libraries are often named after the institution in which they were developed. An example being the RPCI-11 library, which is named after Roswell Park Comprehensive Cancer Center (formerly known as Roswell Park Cancer Institute) in Buffalo, New York. These fragments are on the order of 100 thousand base-pairs, and are the basis for most FISH probes.

Preparation and hybridization process – RNA edit

The purpose of using RNA FISH is to detect target mRNA transcripts in cells, tissue sections, or even whole-mounts.[10] The process is done in 3 main procedures: tissue preparation (pre-hybridization), hybridization, and washing (post-hybridization).

The tissue preparation starts by collecting the appropriate tissue sections to perform RNA FISH. First, cells, circulating tumor cells (CTCs), formalin-fixed paraffin-embedded (FFPE), or frozen tissue sections are fixed. Some commonly used fixatives are 4% formaldehyde or paraformaldehyde (PFA) in phosphate buffered saline (PBS).[10] FISH has also been successfully done on unfixed cells.[11] After fixation, samples are permeabilized to allow the penetration of hybridization reagents. The use of detergents at a 0.1% concentration is commonly used to enhance the tissue permeability such as Tween-20 or Triton X-100.[12]

It is critical for the hybridization process to have all optimal conditions to have a successful in situ result, including temperature, pH, salt concentration, and time of the hybridization reaction. After checking all the necessary conditions, hybridization steps can be started by first adding a target-specific probe, composed of 20 oligonucleotide pairs, hybridizes to the target RNA(s). Separate but compatible signal amplification systems enable the multiplex assay (up to two targets per assay). Signal amplification is achieved via series of sequential hybridization steps.[13]

After the hybridization steps, washing steps are performed. These steps aim to remove nonspecific hybrids and get rid of unbound probe molecules from the samples to reduce any background signaling. The use of ethanol washes are typically used at this stage to reduce autofluorescence in tissues or cells.[14] At the end of the assay the tissue samples are visualized under a fluorescence microscope such as the confocal fluorescence microscope and the Keyence microscope.[12]

Preparation and hybridization process – DNA edit

 
Scheme of the principle of the FISH Experiment to localize a gene in the nucleus.

First, a probe is constructed. The probe must be large enough to hybridize specifically with its target but not so large as to impede the hybridization process. The probe is tagged directly with fluorophores, with targets for antibodies or with biotin. Tagging can be done in various ways, such as nick translation, or polymerase chain reaction using tagged nucleotides.

Then, an interphase or metaphase chromosome preparation is produced. The chromosomes are firmly attached to a substrate, usually glass. Repetitive DNA sequences must be blocked by adding short fragments of DNA to the sample. The probe is then applied to the chromosome DNA and incubated for approximately 12 hours while hybridizing. Several wash steps remove all unhybridized or partially hybridized probes. The results are then visualized and quantified using a microscope that is capable of exciting the dye and recording images.

If the fluorescent signal is weak, amplification of the signal may be necessary in order to exceed the detection threshold of the microscope. Fluorescent signal strength depends on many factors such as probe labeling efficiency, the type of probe, and the type of dye. Fluorescently tagged antibodies or streptavidin are bound to the dye molecule. These secondary components are selected so that they have a strong signal.

Variations on probes and analysis edit

FISH is a very general technique. The differences between the various FISH techniques are usually due to variations in the sequence and labeling of the probes; and how they are used in combination. Probes are divided into two generic categories: cellular and acellular. In fluorescent "in situ" hybridization refers to the cellular placement of the probe

Probe size is important because shorter probes hybridize less specifically than longer probes, so that long enough strands of DNA or RNA (often 10–25 nucleotides) which are complementary to a given target sequence are often used to locate a target. The overlap defines the resolution of detectable features. For example, if the goal of an experiment is to detect the breakpoint of a translocation, then the overlap of the probes — the degree to which one DNA sequence is contained in the adjacent probes — defines the minimum window in which the breakpoint may be detected.

The mixture of probe sequences determines the type of feature the probe can detect. Probes that hybridize along an entire chromosome are used to count the number of a certain chromosome, show translocations, or identify extra-chromosomal fragments of chromatin. This is often called "whole-chromosome painting." If every possible probe is used, every chromosome, (the whole genome) would be marked fluorescently, which would not be particularly useful for determining features of individual sequences. However, it is possible to create a mixture of smaller probes that are specific to a particular region (locus) of DNA; these mixtures are used to detect deletion mutations. When combined with a specific color, a locus-specific probe mixture is used to detect very specific translocations. Special locus-specific probe mixtures are often used to count chromosomes, by binding to the centromeric regions of chromosomes, which are distinctive enough to identify each chromosome (with the exception of Chromosome 13, 14, 21, 22.)

A variety of other techniques uses mixtures of differently colored probes. A range of colors in mixtures of fluorescent dyes can be detected, so each human chromosome can be identified by a characteristic color using whole-chromosome probe mixtures and a variety of ratios of colors. Although there are more chromosomes than easily distinguishable fluorescent dye colors, ratios of probe mixtures can be used to create secondary colors. Similar to comparative genomic hybridization, the probe mixture for the secondary colors is created by mixing the correct ratio of two sets of differently colored probes for the same chromosome. This technique is sometimes called M-FISH.

The same physics that make a variety of colors possible for M-FISH can be used for the detection of translocations. That is, colors that are adjacent appear to overlap; a secondary color is observed. Some assays are designed so that the secondary color will be present or absent in cases of interest. An example is the detection of BCR/ABL translocations, where the secondary color indicates disease. This variation is often called double-fusion FISH or D-FISH. In the opposite situation—where the absence of the secondary color is pathological—is illustrated by an assay used to investigate translocations where only one of the breakpoints is known or constant. Locus-specific probes are made for one side of the breakpoint and the other intact chromosome. In normal cells, the secondary color is observed, but only the primary colors are observed when the translocation occurs. This technique is sometimes called "break-apart FISH".

Single-molecule RNA FISH edit

Single-molecule RNA FISH, also known as Stellaris® RNA FISH[15] or smFISH,[16] is a method of detecting and quantifying mRNA and other long RNA molecules in a thin layer of tissue sample. Targets can be reliably imaged through the application of multiple short singly labeled oligonucleotide probes.[17] The binding of up to 48 fluorescent labeled oligos to a single molecule of mRNA provides sufficient fluorescence to accurately detect and localize each target mRNA in a wide-field fluorescent microscopy image. Probes not binding to the intended sequence do not achieve sufficient localized fluorescence to be distinguished from background.[18]

Single-molecule RNA FISH assays can be performed in simplex or multiplex, and can be used as a follow-up experiment to quantitative PCR, or imaged simultaneously with a fluorescent antibody assay. The technology has potential applications in cancer diagnosis,[19] neuroscience, gene expression analysis,[20] and companion diagnostics.

Fiber FISH edit

In an alternative technique to interphase or metaphase preparations, fiber FISH, interphase chromosomes are attached to a slide in such a way that they are stretched out in a straight line, rather than being tightly coiled, as in conventional FISH, or adopting a chromosome territory conformation, as in interphase FISH. This is accomplished by applying mechanical shear along the length of the slide, either to cells that have been fixed to the slide and then lysed, or to a solution of purified DNA. A technique known as chromosome combing is increasingly used for this purpose. The extended conformation of the chromosomes allows dramatically higher resolution – even down to a few kilobases. The preparation of fiber FISH samples, although conceptually simple, is a rather skilled art, and only specialized laboratories use the technique routinely.[21]

Q-FISH edit

Main article: Q-FISH

Q-FISH combines FISH with PNAs and computer software to quantify fluorescence intensity. This technique is used routinely in telomere length research.

Flow-FISH edit

Main article: Flow-FISH

Flow-FISH uses flow cytometry to perform FISH automatically using per-cell fluorescence measurements.

MA-FISH edit

Microfluidics-assisted FISH (MA-FISH) uses a microfluidic flow to increase DNA hybridization efficiency, decreasing expensive FISH probe consumption and reduce the hybridization time. MA-FISH is applied for detecting the HER2 gene in breast cancer tissues.[22]

MAR-FISH edit

Microautoradiography FISH is a technique to combine radio-labeled substrates with conventional FISH to detect phylogenetic groups and metabolic activities simultaneously.[23]

Hybrid Fusion-FISH edit

Hybrid Fusion FISH (HF-FISH) uses primary additive excitation/emission combination of fluorophores to generate additional spectra through a labeling process known as dynamic optical transmission (DOT). Three primary fluorophores are able to generate a total of 7 readily detectable emission spectra as a result of combinatorial labeling using DOT. Hybrid Fusion FISH enables highly multiplexed FISH applications that are targeted within clinical oncology panels. The technology offers faster scoring with efficient probesets that can be readily detected with traditional fluorescent microscopes.

MERFISH edit

Multiplexed error-robust fluorescence in situ hybridization[24] is a highly multiplexed version of smFISH. It uses combinatorial labeling, followed by imaging, and then error-resistant encoding[25] to capture a high number of RNA molecules and spatial localization within the cell. The capture of a large number of RNA molecules enables elucidation of gene regulatory networks, prediction of function of unannotated genes, and identification of RNA molecule distribution patterns, which correlate with their associated proteins.

STARFISH edit

Starfish is a set of software tools developed in 2019 by a consortium of scientists to analyze data from nine different variations of FISH, since all variations produce the same set of data—gene expression values mapped to x and y coordinates in a cell. The software, created for all scientists, not just bioinformaticians, reads a set of images, removes noise, and identifies RNA molecules. This approach has set out to define a standard analysis scheme of FISH datasets in a similar way to single-cell transcriptomics analysis.[26]

Medical applications edit

Often parents of children with a developmental disability want to know more about their child's conditions before choosing to have another child. These concerns can be addressed by analysis of the parents' and child's DNA. In cases where the child's developmental disability is not understood, the cause of it can potentially be determined using FISH and cytogenetic techniques. Examples of diseases that are diagnosed using FISH include Prader-Willi syndrome, Angelman syndrome, 22q13 deletion syndrome, chronic myelogenous leukemia, acute lymphoblastic leukemia, Cri-du-chat, Velocardiofacial syndrome, and Down syndrome. FISH on sperm cells is indicated for men with an abnormal somatic or meiotic karyotype as well as those with oligozoospermia, since approximately 50% of oligozoospermic men have an increased rate of sperm chromosome abnormalities.[27] The analysis of chromosomes 21, X, and Y is enough to identify oligozoospermic individuals at risk.[27]

In medicine, FISH can be used to form a diagnosis, to evaluate prognosis, or to evaluate remission of a disease, such as cancer. Treatment can then be specifically tailored. A traditional exam involving metaphase chromosome analysis is often unable to identify features that distinguish one disease from another, due to subtle chromosomal features; FISH can elucidate these differences. FISH can also be used to detect diseased cells more easily than standard Cytogenetic methods, which require dividing cells and requires labor and time-intensive manual preparation and analysis of the slides by a technologist. FISH, on the other hand, does not require living cells and can be quantified automatically, a computer counts the fluorescent dots present. However, a trained technologist is required to distinguish subtle differences in banding patterns on bent and twisted metaphase chromosomes. FISH can be incorporated into Lab-on-a-chip microfluidic device. This technology is still in a developmental stage but, like other lab on a chip methods, it may lead to more portable diagnostic techniques.[28][29]

 
General process of fluorescent in situ hybridization (FISH) used for bacterial pathogen identification. First, an infected tissue sample is taken from the patient. Then an oligonucleotide complementary to the suspected pathogen's genetic code is chemically tagged with a fluorescent probe. The tissue sample is chemically treated in order to make the cell membranes permeable to the fluorescently tagged oligonucleotide. The fluorescent tag is then added and only binds to the complementary DNA of the suspected pathogen. If the pathogen is present in the tissue sample, then the pathogen's cells will fluoresce after treatment with the tagged oligonucleotide. No other cells will glow.

Species identification edit

FISH has been extensively studied as a diagnostic technique for the identification of pathogens in the field of medical microbiology.[30] Although it has been proven to be a useful and applicable technique, it is still not widely applied in diagnostic laboratories. The short time to diagnosis (less than 2 hours) has been a major advantage compared with biochemical differentiation, but this advantage is challenged by MALDI-TOF-MS which allows the identification of a wider range of pathogens compared with biochemical differentiation techniques. Using FISH for diagnostic purposes has found its purpose when immediate species identification is needed, specifically for the investigation of blood cultures for which FISH is a cheap and easy technique for preliminary rapid diagnosis.[30]

FISH can also be used to compare the genomes of two biological species, to deduce evolutionary relationships. A similar hybridization technique is called a zoo blot. Bacterial FISH probes are often primers for the 16s rRNA region.

FISH is widely used in the field of microbial ecology, to identify microorganisms. Biofilms, for example, are composed of complex (often) multi-species bacterial organizations. Preparing DNA probes for one species and performing FISH with this probe allows one to visualize the distribution of this specific species within the biofilm. Preparing probes (in two different colors) for two species allows researchers to visualize/study co-localization of these two species in the biofilm and can be useful in determining the fine architecture of the biofilm.

Comparative genomic hybridization edit

Comparative genomic hybridization can be described as a method that uses FISH in a parallel manner with the comparison of the hybridization strength to recall any major disruptions in the duplication process of the DNA sequences in the genome of the nucleus.[31]

Virtual karyotype edit

Virtual karyotyping is another cost-effective, clinically available alternative to FISH panels using thousands to millions of probes on a single array to detect copy number changes, genome-wide, at unprecedented resolution. Currently, this type of analysis will only detect gains and losses of chromosomal material and will not detect balanced rearrangements, such as translocations and inversions which are hallmark aberrations seen in many types of leukemia and lymphoma.

Spectral karyotype edit

Spectral karyotyping is an image of colored chromosomes. Spectral karyotyping involves FISH using multiple forms of many types of probes with the result to see each chromosome labeled through its metaphase stage. This type of karyotyping is used specifically when seeking out chromosome arrangements.

Chromosome evolution edit

 
Human chromosomes painted with DNA from mouse chromosome 11 showing hybridization signals on human chromosomes 17, 5, 2, 7, and 22 and some other chromosomes. That is, an ancestral chromosome broke up into multiple fragments that can still be found in many human chromosomes.[32]

FISH can be used to study the evolution of chromosomes. Species that are related have similar chromosomes. This homology can be detected by gene or genome sequencing but also by FISH. For instance, human and chimpanzee chromosomes are very similar and FISH can demonstrate that two chimpanzee chromosomes fused to result in one human chromosome. Similarly, species that are more distantly related, have similar chromosomes but with increasing distance chromosomes tend to break and fuse and thus result in mosaic chromosomes. This can be impressively demonstrated by FISH (see figure).[32]

See also edit

Gallery edit

  •  
    Another schematic of FISH process.
  •  
    Microfluidic chip that lowered the cost-per-test of FISH by 90%.
  •  
    Dual label FISH image; Bifidobacteria Cy3, Total bacteria FITC.
  •  
    Paraspeckles visualized by single-molecule FISH against NEAT1 (Quasar 570) in U-2 OS cells (DAPI).

References edit

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Further reading edit

  • Pernthaler A, Pernthaler J, Amann R (June 2002). "Fluorescence in situ hybridization and catalyzed reporter deposition for the identification of marine bacteria". Applied and Environmental Microbiology. 68 (6): 3094–3101. Bibcode:2002ApEnM..68.3094P. doi:10.1128/AEM.68.6.3094-3101.2002. PMC 123953. PMID 12039771.
  • Wagner M, Horn M, Daims H (June 2003). "Fluorescence in situ hybridisation for the identification and characterisation of prokaryotes". Current Opinion in Microbiology. 6 (3): 302–309. doi:10.1016/S1369-5274(03)00054-7. PMID 12831908.
  • Carthy JD (1965). Viewpoints In Biology. England: Butterworth & Co. p. 66.

External links edit

 
Wikimedia Commons has media related to Fluorescence in situ hybridization.
  • Fluorescent+in+Situ+Hybridization at the U.S. National Library of Medicine Medical Subject Headings (MeSH)
  • Information on from the Olympus Corporation
  • A guide to fiber FISH from Octavian Henegariu
  • Fibre FISH protocol 2006-10-23 at the Wayback Machine from the Human Genome Project at the Sanger Centre
  • CARD-FISH, BioMineWiki 2020-07-28 at the Wayback Machine
  • Preparation of Complex DNA Probe Sets for 3D FISH with up to Six Different Fluorochromes
  • FISH technical notes and protocols from GeneDetect.com
  • Fluorescence in situ Hybridization Photos of bacteria 2015-02-05 at the Wayback Machine
  • Rational design of polynucleotide probe mixes to identify particular genes in defined taxa: www.dnaBaser.com/PolyPro

January 01, 1970
fluorescence, situ, hybridization, fish, molecular, cytogenetic, technique, that, uses, fluorescent, probes, that, bind, only, particular, parts, nucleic, acid, sequence, with, high, degree, sequence, complementarity, developed, biomedical, researchers, early,. Fluorescence in situ hybridization FISH is a molecular cytogenetic technique that uses fluorescent probes that bind to only particular parts of a nucleic acid sequence with a high degree of sequence complementarity It was developed by biomedical researchers in the early 1980s 1 to detect and localize the presence or absence of specific DNA sequences on chromosomes Fluorescence microscopy can be used to find out where the fluorescent probe is bound to the chromosomes FISH is often used for finding specific features in DNA for use in genetic counseling medicine and species identification 2 FISH can also be used to detect and localize specific RNA targets mRNA lncRNA and miRNA citation needed in cells circulating tumor cells and tissue samples In this context it can help define the spatial temporal patterns of gene expression within cells and tissues Multiplex RNA visualization in cells using ViewRNA FISH Assays A metaphase cell positive for the bcr abl rearrangement associated with chronic myelogenous leukemia using FISH The chromosomes can be seen in blue The chromosome that is labeled with green and red spots upper left is the one where the rearrangement is present Contents 1 Probes RNA and DNA 1 1 Preparation and hybridization process RNA 1 2 Preparation and hybridization process DNA 2 Variations on probes and analysis 2 1 Single molecule RNA FISH 2 2 Fiber FISH 2 3 Q FISH 2 4 Flow FISH 2 5 MA FISH 2 6 MAR FISH 2 7 Hybrid Fusion FISH 2 8 MERFISH 2 9 STARFISH 3 Medical applications 3 1 Species identification 3 2 Comparative genomic hybridization 3 3 Virtual karyotype 3 4 Spectral karyotype 4 Chromosome evolution 5 See also 6 Gallery 7 References 8 Further reading 9 External linksProbes RNA and DNA edit nbsp ViewRNA detection of miR 133 green and myogenin mRNA red in C2C12 differentiating cells In biology a probe is a single strand of DNA or RNA that is complementary to a nucleotide sequence of interest RNA probes can be designed for any gene or any sequence within a gene for visualization of mRNA 3 4 5 lncRNA 6 7 8 and miRNA in tissues and cells FISH is used by examining the cellular reproduction cycle specifically interphase of the nuclei for any chromosomal abnormalities 9 FISH allows the analysis of a large series of archival cases much easier to identify the pinpointed chromosome by creating a probe with an artificial chromosomal foundation that will attract similar chromosomes 9 The hybridization signals for each probe when a nucleic abnormality is detected 9 Each probe for the detection of mRNA and lncRNA is composed of 20 50 oligonucleotide pairs each pair covering a space of 40 50 bp The specifics depend on the specific FISH technique used For miRNA detection the probes use proprietary chemistry for specific detection of miRNA and cover the entire miRNA sequence nbsp Urothelial cells marked with four different probes Probes are often derived from fragments of DNA that were isolated purified and amplified for use in the Human Genome Project The size of the human genome is so large compared to the length that could be sequenced directly that it was necessary to divide the genome into fragments In the eventual analysis these fragments were put into order by digesting a copy of each fragment into still smaller fragments using sequence specific endonucleases measuring the size of each small fragment using size exclusion chromatography and using that information to determine where the large fragments overlapped one another To preserve the fragments with their individual DNA sequences the fragments were added into a system of continually replicating bacteria populations Clonal populations of bacteria each population maintaining a single artificial chromosome are stored in various laboratories around the world The artificial chromosomes BAC can be grown extracted and labeled in any lab containing a library Genomic libraries are often named after the institution in which they were developed An example being the RPCI 11 library which is named after Roswell Park Comprehensive Cancer Center formerly known as Roswell Park Cancer Institute in Buffalo New York These fragments are on the order of 100 thousand base pairs and are the basis for most FISH probes Preparation and hybridization process RNA edit The purpose of using RNA FISH is to detect target mRNA transcripts in cells tissue sections or even whole mounts 10 The process is done in 3 main procedures tissue preparation pre hybridization hybridization and washing post hybridization The tissue preparation starts by collecting the appropriate tissue sections to perform RNA FISH First cells circulating tumor cells CTCs formalin fixed paraffin embedded FFPE or frozen tissue sections are fixed Some commonly used fixatives are 4 formaldehyde or paraformaldehyde PFA in phosphate buffered saline PBS 10 FISH has also been successfully done on unfixed cells 11 After fixation samples are permeabilized to allow the penetration of hybridization reagents The use of detergents at a 0 1 concentration is commonly used to enhance the tissue permeability such as Tween 20 or Triton X 100 12 It is critical for the hybridization process to have all optimal conditions to have a successful in situ result including temperature pH salt concentration and time of the hybridization reaction After checking all the necessary conditions hybridization steps can be started by first adding a target specific probe composed of 20 oligonucleotide pairs hybridizes to the target RNA s Separate but compatible signal amplification systems enable the multiplex assay up to two targets per assay Signal amplification is achieved via series of sequential hybridization steps 13 After the hybridization steps washing steps are performed These steps aim to remove nonspecific hybrids and get rid of unbound probe molecules from the samples to reduce any background signaling The use of ethanol washes are typically used at this stage to reduce autofluorescence in tissues or cells 14 At the end of the assay the tissue samples are visualized under a fluorescence microscope such as the confocal fluorescence microscope and the Keyence microscope 12 Preparation and hybridization process DNA edit nbsp Scheme of the principle of the FISH Experiment to localize a gene in the nucleus First a probe is constructed The probe must be large enough to hybridize specifically with its target but not so large as to impede the hybridization process The probe is tagged directly with fluorophores with targets for antibodies or with biotin Tagging can be done in various ways such as nick translation or polymerase chain reaction using tagged nucleotides Then an interphase or metaphase chromosome preparation is produced The chromosomes are firmly attached to a substrate usually glass Repetitive DNA sequences must be blocked by adding short fragments of DNA to the sample The probe is then applied to the chromosome DNA and incubated for approximately 12 hours while hybridizing Several wash steps remove all unhybridized or partially hybridized probes The results are then visualized and quantified using a microscope that is capable of exciting the dye and recording images If the fluorescent signal is weak amplification of the signal may be necessary in order to exceed the detection threshold of the microscope Fluorescent signal strength depends on many factors such as probe labeling efficiency the type of probe and the type of dye Fluorescently tagged antibodies or streptavidin are bound to the dye molecule These secondary components are selected so that they have a strong signal Variations on probes and analysis editFISH is a very general technique The differences between the various FISH techniques are usually due to variations in the sequence and labeling of the probes and how they are used in combination Probes are divided into two generic categories cellular and acellular In fluorescent in situ hybridization refers to the cellular placement of the probeProbe size is important because shorter probes hybridize less specifically than longer probes so that long enough strands of DNA or RNA often 10 25 nucleotides which are complementary to a given target sequence are often used to locate a target The overlap defines the resolution of detectable features For example if the goal of an experiment is to detect the breakpoint of a translocation then the overlap of the probes the degree to which one DNA sequence is contained in the adjacent probes defines the minimum window in which the breakpoint may be detected The mixture of probe sequences determines the type of feature the probe can detect Probes that hybridize along an entire chromosome are used to count the number of a certain chromosome show translocations or identify extra chromosomal fragments of chromatin This is often called whole chromosome painting If every possible probe is used every chromosome the whole genome would be marked fluorescently which would not be particularly useful for determining features of individual sequences However it is possible to create a mixture of smaller probes that are specific to a particular region locus of DNA these mixtures are used to detect deletion mutations When combined with a specific color a locus specific probe mixture is used to detect very specific translocations Special locus specific probe mixtures are often used to count chromosomes by binding to the centromeric regions of chromosomes which are distinctive enough to identify each chromosome with the exception of Chromosome 13 14 21 22 A variety of other techniques uses mixtures of differently colored probes A range of colors in mixtures of fluorescent dyes can be detected so each human chromosome can be identified by a characteristic color using whole chromosome probe mixtures and a variety of ratios of colors Although there are more chromosomes than easily distinguishable fluorescent dye colors ratios of probe mixtures can be used to create secondary colors Similar to comparative genomic hybridization the probe mixture for the secondary colors is created by mixing the correct ratio of two sets of differently colored probes for the same chromosome This technique is sometimes called M FISH The same physics that make a variety of colors possible for M FISH can be used for the detection of translocations That is colors that are adjacent appear to overlap a secondary color is observed Some assays are designed so that the secondary color will be present or absent in cases of interest An example is the detection of BCR ABL translocations where the secondary color indicates disease This variation is often called double fusion FISH or D FISH In the opposite situation where the absence of the secondary color is pathological is illustrated by an assay used to investigate translocations where only one of the breakpoints is known or constant Locus specific probes are made for one side of the breakpoint and the other intact chromosome In normal cells the secondary color is observed but only the primary colors are observed when the translocation occurs This technique is sometimes called break apart FISH Single molecule RNA FISH edit Single molecule RNA FISH also known as Stellaris RNA FISH 15 or smFISH 16 is a method of detecting and quantifying mRNA and other long RNA molecules in a thin layer of tissue sample Targets can be reliably imaged through the application of multiple short singly labeled oligonucleotide probes 17 The binding of up to 48 fluorescent labeled oligos to a single molecule of mRNA provides sufficient fluorescence to accurately detect and localize each target mRNA in a wide field fluorescent microscopy image Probes not binding to the intended sequence do not achieve sufficient localized fluorescence to be distinguished from background 18 Single molecule RNA FISH assays can be performed in simplex or multiplex and can be used as a follow up experiment to quantitative PCR or imaged simultaneously with a fluorescent antibody assay The technology has potential applications in cancer diagnosis 19 neuroscience gene expression analysis 20 and companion diagnostics Fiber FISH edit In an alternative technique to interphase or metaphase preparations fiber FISH interphase chromosomes are attached to a slide in such a way that they are stretched out in a straight line rather than being tightly coiled as in conventional FISH or adopting a chromosome territory conformation as in interphase FISH This is accomplished by applying mechanical shear along the length of the slide either to cells that have been fixed to the slide and then lysed or to a solution of purified DNA A technique known as chromosome combing is increasingly used for this purpose The extended conformation of the chromosomes allows dramatically higher resolution even down to a few kilobases The preparation of fiber FISH samples although conceptually simple is a rather skilled art and only specialized laboratories use the technique routinely 21 Q FISH edit Main article Q FISH Q FISH combines FISH with PNAs and computer software to quantify fluorescence intensity This technique is used routinely in telomere length research Flow FISH edit Main article Flow FISH Flow FISH uses flow cytometry to perform FISH automatically using per cell fluorescence measurements MA FISH edit Microfluidics assisted FISH MA FISH uses a microfluidic flow to increase DNA hybridization efficiency decreasing expensive FISH probe consumption and reduce the hybridization time MA FISH is applied for detecting the HER2 gene in breast cancer tissues 22 MAR FISH edit Microautoradiography FISH is a technique to combine radio labeled substrates with conventional FISH to detect phylogenetic groups and metabolic activities simultaneously 23 Hybrid Fusion FISH edit Hybrid Fusion FISH HF FISH uses primary additive excitation emission combination of fluorophores to generate additional spectra through a labeling process known as dynamic optical transmission DOT Three primary fluorophores are able to generate a total of 7 readily detectable emission spectra as a result of combinatorial labeling using DOT Hybrid Fusion FISH enables highly multiplexed FISH applications that are targeted within clinical oncology panels The technology offers faster scoring with efficient probesets that can be readily detected with traditional fluorescent microscopes MERFISH edit Multiplexed error robust fluorescence in situ hybridization 24 is a highly multiplexed version of smFISH It uses combinatorial labeling followed by imaging and then error resistant encoding 25 to capture a high number of RNA molecules and spatial localization within the cell The capture of a large number of RNA molecules enables elucidation of gene regulatory networks prediction of function of unannotated genes and identification of RNA molecule distribution patterns which correlate with their associated proteins STARFISH edit Starfish is a set of software tools developed in 2019 by a consortium of scientists to analyze data from nine different variations of FISH since all variations produce the same set of data gene expression values mapped to x and y coordinates in a cell The software created for all scientists not just bioinformaticians reads a set of images removes noise and identifies RNA molecules This approach has set out to define a standard analysis scheme of FISH datasets in a similar way to single cell transcriptomics analysis 26 Medical applications editOften parents of children with a developmental disability want to know more about their child s conditions before choosing to have another child These concerns can be addressed by analysis of the parents and child s DNA In cases where the child s developmental disability is not understood the cause of it can potentially be determined using FISH and cytogenetic techniques Examples of diseases that are diagnosed using FISH include Prader Willi syndrome Angelman syndrome 22q13 deletion syndrome chronic myelogenous leukemia acute lymphoblastic leukemia Cri du chat Velocardiofacial syndrome and Down syndrome FISH on sperm cells is indicated for men with an abnormal somatic or meiotic karyotype as well as those with oligozoospermia since approximately 50 of oligozoospermic men have an increased rate of sperm chromosome abnormalities 27 The analysis of chromosomes 21 X and Y is enough to identify oligozoospermic individuals at risk 27 In medicine FISH can be used to form a diagnosis to evaluate prognosis or to evaluate remission of a disease such as cancer Treatment can then be specifically tailored A traditional exam involving metaphase chromosome analysis is often unable to identify features that distinguish one disease from another due to subtle chromosomal features FISH can elucidate these differences FISH can also be used to detect diseased cells more easily than standard Cytogenetic methods which require dividing cells and requires labor and time intensive manual preparation and analysis of the slides by a technologist FISH on the other hand does not require living cells and can be quantified automatically a computer counts the fluorescent dots present However a trained technologist is required to distinguish subtle differences in banding patterns on bent and twisted metaphase chromosomes FISH can be incorporated into Lab on a chip microfluidic device This technology is still in a developmental stage but like other lab on a chip methods it may lead to more portable diagnostic techniques 28 29 nbsp General process of fluorescent in situ hybridization FISH used for bacterial pathogen identification First an infected tissue sample is taken from the patient Then an oligonucleotide complementary to the suspected pathogen s genetic code is chemically tagged with a fluorescent probe The tissue sample is chemically treated in order to make the cell membranes permeable to the fluorescently tagged oligonucleotide The fluorescent tag is then added and only binds to the complementary DNA of the suspected pathogen If the pathogen is present in the tissue sample then the pathogen s cells will fluoresce after treatment with the tagged oligonucleotide No other cells will glow Species identification edit FISH has been extensively studied as a diagnostic technique for the identification of pathogens in the field of medical microbiology 30 Although it has been proven to be a useful and applicable technique it is still not widely applied in diagnostic laboratories The short time to diagnosis less than 2 hours has been a major advantage compared with biochemical differentiation but this advantage is challenged by MALDI TOF MS which allows the identification of a wider range of pathogens compared with biochemical differentiation techniques Using FISH for diagnostic purposes has found its purpose when immediate species identification is needed specifically for the investigation of blood cultures for which FISH is a cheap and easy technique for preliminary rapid diagnosis 30 FISH can also be used to compare the genomes of two biological species to deduce evolutionary relationships A similar hybridization technique is called a zoo blot Bacterial FISH probes are often primers for the 16s rRNA region FISH is widely used in the field of microbial ecology to identify microorganisms Biofilms for example are composed of complex often multi species bacterial organizations Preparing DNA probes for one species and performing FISH with this probe allows one to visualize the distribution of this specific species within the biofilm Preparing probes in two different colors for two species allows researchers to visualize study co localization of these two species in the biofilm and can be useful in determining the fine architecture of the biofilm Comparative genomic hybridization edit Comparative genomic hybridization can be described as a method that uses FISH in a parallel manner with the comparison of the hybridization strength to recall any major disruptions in the duplication process of the DNA sequences in the genome of the nucleus 31 Virtual karyotype edit Virtual karyotyping is another cost effective clinically available alternative to FISH panels using thousands to millions of probes on a single array to detect copy number changes genome wide at unprecedented resolution Currently this type of analysis will only detect gains and losses of chromosomal material and will not detect balanced rearrangements such as translocations and inversions which are hallmark aberrations seen in many types of leukemia and lymphoma Spectral karyotype edit Spectral karyotyping is an image of colored chromosomes Spectral karyotyping involves FISH using multiple forms of many types of probes with the result to see each chromosome labeled through its metaphase stage This type of karyotyping is used specifically when seeking out chromosome arrangements Chromosome evolution edit nbsp Human chromosomes painted with DNA from mouse chromosome 11 showing hybridization signals on human chromosomes 17 5 2 7 and 22 and some other chromosomes That is an ancestral chromosome broke up into multiple fragments that can still be found in many human chromosomes 32 FISH can be used to study the evolution of chromosomes Species that are related have similar chromosomes This homology can be detected by gene or genome sequencing but also by FISH For instance human and chimpanzee chromosomes are very similar and FISH can demonstrate that two chimpanzee chromosomes fused to result in one human chromosome Similarly species that are more distantly related have similar chromosomes but with increasing distance chromosomes tend to break and fuse and thus result in mosaic chromosomes This can be impressively demonstrated by FISH see figure 32 See also editChromogenic in situ hybridization CISH Eukaryotic chromosome fine structure G banding Gene mapping Genome evolution Happy mapping In situ hybridization the technique used for labelling Molecular cytogenetics Virtual karyotypeGallery edit nbsp Another schematic of FISH process nbsp Microfluidic chip that lowered the cost per test of FISH by 90 nbsp Dual label FISH image Bifidobacteria Cy3 Total bacteria FITC nbsp Paraspeckles visualized by single molecule FISH against NEAT1 Quasar 570 in U 2 OS cells DAPI References edit Langer Safer PR Levine M Ward DC July 1982 Immunological method for mapping genes on Drosophila polytene chromosomes Proceedings of the National Academy of Sciences of the United States of America 79 14 4381 4385 Bibcode 1982PNAS 79 4381L doi 10 1073 pnas 79 14 4381 PMC 346675 PMID 6812046 Amann R Fuchs BM May 2008 Single cell identification in microbial communities by improved fluorescence in situ hybridization techniques Nature Reviews Microbiology 6 5 339 348 doi 10 1038 nrmicro1888 PMID 18414500 S2CID 22498325 Anthony SJ St Leger JA Pugliares K Ip HS Chan JM Carpenter ZW et al 2012 Emergence of fatal avian influenza in New England harbor seals mBio 3 4 e00166 e00112 doi 10 1128 mBio 00166 12 PMC 3419516 PMID 22851656 Everitt AR Clare S Pertel T John SP Wash RS Smith SE et al March 2012 IFITM3 restricts the morbidity and mortality associated with influenza Nature 484 7395 519 523 Bibcode 2012Natur 484 519 doi 10 1038 nature10921 PMC 3648786 PMID 22446628 Louzada S Adega F Chaves R 2012 Defining the sister rat mammary tumor cell lines HH 16 cl 2 1 and HH 16 cl 4 as an in vitro cell model for Erbb2 PLOS ONE 7 1 e29923 Bibcode 2012PLoSO 729923L doi 10 1371 journal pone 0029923 PMC 3254647 PMID 22253826 Ting DT Lipson D Paul S Brannigan BW Akhavanfard S Coffman EJ et al February 2011 Aberrant overexpression of satellite repeats in pancreatic and other epithelial cancers Science 331 6017 593 596 Bibcode 2011Sci 331 593T doi 10 1126 science 1200801 PMC 3701432 PMID 21233348 Zhang B Arun G Mao YS Lazar Z Hung G Bhattacharjee G et al July 2012 The lncRNA Malat1 is dispensable for mouse development but its transcription plays a cis regulatory role in the adult Cell Reports 2 1 111 123 doi 10 1016 j celrep 2012 06 003 PMC 3408587 PMID 22840402 Lee K Kunkeaw N Jeon SH Lee I Johnson BH Kang GY et al June 2011 Precursor miR 886 a novel noncoding RNA repressed in cancer associates with PKR and modulates its activity RNA 17 6 1076 1089 doi 10 1261 rna 2701111 PMC 3096040 PMID 21518807 a b c Bernasconi B Karamitopoulou Diamantis E Karamitopolou Diamantiis E Tornillo L Lugli A Di Vizio D et al April 2008 Chromosomal instability in gastric mucosa associated lymphoid tissue lymphomas a fluorescent in situ hybridization study using a tissue microarray approach Human Pathology 39 4 536 542 doi 10 1016 j humpath 2007 08 009 PMID 18234275 a b Young AP Jackson DJ Wyeth RC 2020 03 19 A technical review and guide to RNA fluorescence in situ hybridization PeerJ 8 e8806 doi 10 7717 peerj 8806 PMC 7085896 PMID 32219032 Haroon MF Skennerton CT Steen JA Lachner N Hugenholtz P Tyson GW 2013 In solution fluorescence in situ hybridization and fluorescence activated cell sorting for single cell and population genome recovery Microbial Metagenomics Metatranscriptomics and Metaproteomics Methods in Enzymology Vol 531 pp 3 19 doi 10 1016 B978 0 12 407863 5 00001 0 ISBN 9780124078635 PMID 24060113 a b Cui C Shu W Li P 2016 Fluorescence In situ Hybridization Cell Based Genetic Diagnostic and Research Applications Frontiers in Cell and Developmental Biology 4 89 doi 10 3389 fcell 2016 00089 PMC 5011256 PMID 27656642 Xie F Timme KA Wood JR May 2018 Using Single Molecule mRNA Fluorescent in Situ Hybridization RNA FISH to Quantify mRNAs in Individual Murine Oocytes and Embryos Scientific Reports 8 1 7930 Bibcode 2018NatSR 8 7930X doi 10 1038 s41598 018 26345 0 PMC 5962540 PMID 29785002 Oliveira VC Carrara RC Simoes DL Saggioro FP Carlotti CG Covas DT Neder L August 2010 Sudan Black B treatment reduces autofluorescence and improves resolution of in situ hybridization specific fluorescent signals of brain sections Histology and Histopathology 25 8 1017 1024 doi 10 14670 HH 25 1017 PMID 20552552 Orjalo AV Johansson HE 2016 01 01 Stellaris RNA Fluorescence in Situ Hybridization for the Simultaneous Detection of Immature and Mature Long Noncoding RNAs in Adherent Cells In Feng Y Zhang L eds Long Non Coding RNAs Methods in Molecular Biology Vol 1402 Springer New York pp 119 134 doi 10 1007 978 1 4939 3378 5 10 ISBN 9781493933761 PMID 26721487 Chen J McSwiggen D Unal E May 2018 Single Molecule Fluorescence In Situ Hybridization smFISH Analysis in Budding Yeast Vegetative Growth and Meiosis Journal of Visualized Experiments 135 doi 10 3791 57774 PMC 6101419 PMID 29889208 Raj A van den Bogaard P Rifkin SA van Oudenaarden A Tyagi S October 2008 Imaging individual mRNA molecules using multiple singly labeled probes Nature Methods 5 10 877 879 doi 10 1038 nmeth 1253 PMC 3126653 PMID 18806792 Biosearch Technologies Signs Exclusive License for Single Molecule FISH Technologies from UMDNJ biosearchtech com Cagir B Gelmann A Park J Fava T Tankelevitch A Bittner EW et al December 1999 Guanylyl cyclase C messenger RNA is a biomarker for recurrent stage II colorectal cancer Annals of Internal Medicine 131 11 805 812 doi 10 7326 0003 4819 131 11 199912070 00024 PMID 10610624 Kosman D Mizutani CM Lemons D Cox WG McGinnis W Bier E August 2004 Multiplex detection of RNA expression in Drosophila embryos Science 305 5685 846 doi 10 1126 science 1099247 PMID 15297669 S2CID 26313219 Heiskanen M Kallioniemi O Palotie A March 1996 Fiber FISH experiences and a refined protocol Genetic Analysis 12 5 6 179 184 doi 10 1016 S1050 3862 96 80004 0 PMID 8740834 Nguyen HT Trouillon R Matsuoka S Fiche M de Leval L Bisig B Gijs MA January 2017 Microfluidics assisted fluorescence in situ hybridization for advantageous human epidermal growth factor receptor 2 assessment in breast cancer Laboratory Investigation A Journal of Technical Methods and Pathology 97 1 93 103 doi 10 1038 labinvest 2016 121 PMID 27892928 Okabe S Kindaichi T Ito T 2004 MAR FISH An Ecophysiological Approach to Link Phylogenetic Affiliation and In Situ Metabolic Activity of Microorganisms at a Single Cell Resolution Microbes and Environments 19 2 83 98 doi 10 1264 jsme2 19 83 Chen KH Boettiger AN Moffitt JR Wang S Zhuang X April 2015 RNA imaging Spatially resolved highly multiplexed RNA profiling in single cells Science 348 6233 aaa6090 doi 10 1126 science aaa6090 PMC 4662681 PMID 25858977 Chen KH Boettiger AN Moffitt JR Wang S Zhuang X April 2015 RNA imaging Spatially resolved highly multiplexed RNA profiling in single cells Science 348 6233 aaa6090 doi 10 1126 science aaa6090 PMC 4662681 PMID 25858977 Perkel JM August 2019 Starfish enterprise finding RNA patterns in single cells Nature 572 7770 549 551 Bibcode 2019Natur 572 549P doi 10 1038 d41586 019 02477 9 PMID 31427807 S2CID 201064966 a b Sarrate Z Vidal F Blanco J April 2010 Role of sperm fluorescent in situ hybridization studies in infertile patients indications study approach and clinical relevance Fertility and Sterility 93 6 1892 1902 doi 10 1016 j fertnstert 2008 12 139 PMID 19254793 Kurz CM Moosdijk SV Thielecke H Velten T 2011 Towards a cellular multi parameter analysis platform Fluorescence in situ hybridization FISH on microhole array chips 2011 Annual International Conference of the IEEE Engineering in Medicine and Biology Society Vol 2011 pp 8408 8411 doi 10 1109 IEMBS 2011 6092074 ISBN 978 1 4577 1589 1 PMID 22256298 S2CID 4955677 Dill K Liu R Grodzinsky P eds 2008 Microarrays Preparation Microfluidics Detection Methods and Biological Applications Springer p 323 ISBN 978 0387727165 a b Frickmann H Zautner AE Moter A Kikhney J Hagen RM Stender H Poppert S May 2017 Fluorescence in situ hybridization FISH in the microbiological diagnostic routine laboratory a review Critical Reviews in Microbiology 43 3 263 293 doi 10 3109 1040841X 2016 1169990 PMID 28129707 S2CID 25252460 Comparative Genomic Hybridization McGraw Hill Dictionary of Scientific and Technical Terms Retrieved September 19 2013 a b Ferguson Smith MA Pereira JC Borges A Kasai F October 2022 Observations on chromosome specific sequencing for the construction of cross species chromosome homology maps and its resolution of human alpaca homology Molecular Cytogenetics 15 1 44 doi 10 1186 s13039 022 00622 0 PMC 9547437 PMID 36207754 Further reading editPernthaler A Pernthaler J Amann R June 2002 Fluorescence in situ hybridization and catalyzed reporter deposition for the identification of marine bacteria Applied and Environmental Microbiology 68 6 3094 3101 Bibcode 2002ApEnM 68 3094P doi 10 1128 AEM 68 6 3094 3101 2002 PMC 123953 PMID 12039771 Wagner M Horn M Daims H June 2003 Fluorescence in situ hybridisation for the identification and characterisation of prokaryotes Current Opinion in Microbiology 6 3 302 309 doi 10 1016 S1369 5274 03 00054 7 PMID 12831908 Carthy JD 1965 Viewpoints In Biology England Butterworth amp Co p 66 External links edit nbsp Wikimedia Commons has media related to Fluorescence in situ hybridization Fluorescent in Situ Hybridization at the U S National Library of Medicine Medical Subject Headings MeSH Information on fiber FISH from the Olympus Corporation A guide to fiber FISH from Octavian Henegariu Fibre FISH protocol Archived 2006 10 23 at the Wayback Machine from the Human Genome Project at the Sanger Centre CARD FISH BioMineWiki Archived 2020 07 28 at the Wayback Machine Preparation of Complex DNA Probe Sets for 3D FISH with up to Six Different Fluorochromes FISH technical notes and protocols from GeneDetect com Fluorescence in situ Hybridization Photos of bacteria Archived 2015 02 05 at the Wayback Machine Rational design of polynucleotide probe mixes to identify particular genes in defined taxa www dnaBaser com PolyPro Retrieved from https en wikipedia org w index php title Fluorescence in situ hybridization amp oldid 1190312206, wikipedia, wiki, book, books, library,

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