Molecular diagnostics Iveta Valaskova Clinical Genetics 22.- 26.11.2021(aZLKG0911s) Outline of the presentation ̶ Application of molecular-genetic testing ̶ Methods used and practical examples Clinical Genetics 22.- 26.11.2021(aZLKG0911s) Aplications of Molecular Genetic Testing • Diagnostic testing Testing for a gene pathological variant in symptomatic individuals as a diagnostic aid Testing requires genetic counseling. • Newborn screening Testing is used to screen populations to identify prevalent genetic pathological variant in asymptomatic infants. The purpose of the screening is to identify affected babies early in life to allow for appropriate intervention before irreversible damage occurs. • Presymptomatic testing Testing for a pathogenic variant in asymptomatic individuals in order to predict or asses the risk of disease in the future. These applications include testing for diseases in which lifestyle changes, increased medical surveillance, or medical intervention might be beneficial if the pathological variant is known. Testing requires extensive pretest and posttest counseling. • Carrier screening Testing for a pathological variant in an autosomal recesive disorder in asymptomatic individuals for the purpose of family planning and genetic counseling to determine probability of disease in childern. Test requires extensive pretest and posttest counseling. • Prenatal diagnosis Testing fetal cells/tissues for mutations to determine if a fetus is affected with a disease early in the pregnancy. Genetic testing, through interrogation of DNA, RNA, can provide critical information for the detection of heritable disease genotypes for a number of different applications Diagnostic testing Classification System for sequence variant identified by genetic testing Newborn screening • Newborn infant has screening tests before leaving the hospital. • There may be different tests depending on the country where you live • Tests on a few drops of blood from pricking the baby's heel. • The tests look for inherited disorders. These tests look for serious medical conditions. If not treated, some of these conditions can cause lifelong health problems. Others can cause early death. With early diagnosis, treatment can begin right away, before serious problems can occur or become permanent. Presymptomatic (predictive) testing This is used in a clinical setting for late-onset conditions such as Huntington disease and familiar cancers. Ideally the family pathogenic variant will have been identified through testing an affected individual. Predictive testing needs to be done within the context of detailed written protocols that define in advance the response to each possible outcome and allow individuals to have adequate information on which to base their decision about whether to proceed to testing. Carrier screening This is used for autosomal and X-linked recessive conditions (and also for balanced chromosomal abnormalities. It would normally be carried out at the request of the patient, and for a reason beyond mere curiosity. Might be recommended in various situations including 1. If one or both partners have a family history of disease 2. If one or both partners are members of a population or ethnic group with a higher incidence of the disease 3. If partners are seeking preconception or prenatal testing 4. General population screening Counseling should always be part of the process, though when testing is done as a part of a population screening program. Pre-test counseling is likely to be quite minimal. Children should not be tested unless there is an immediate benefit to the child. Prenatal diagnosis Prenatal diagnosis means diagnosis before birth. It’s a way to see if developing baby has a problem. These tests help find genetic disorders before birth. Some parents have increased risk of having a baby with a genetic disorder or other problem. Knowing about problems before the baby is born may help parents. They may be able to make better decisions about health care for their infant. Certain problems can be treated before the baby is born. Other problems may need special treatment right after delivery. In some cases, parents may even decide not to continue the pregnancy. Prenatal diagnosis A comparative schematic of prenatal diagnostic techniques and their applicability with respect to the progress of pregnancy: • conventional invasive procedures (amniocentesis, chorionic villi sampling); Testing can be done at 11 to 13 wk gestation by chorionic villus sampling (CVS) or at 14-20 wk by amniocentesis. • serum screening techniques (triple and quad screens - ultrasonography); • non-invasive prenatal diagnostics (cell-free fetal DNA sampling methods). This can be carried out at several stages of pregnancy Chaitanya Kantak, Chia-Pin Chang, Chee Chung Wong, Aniza Mahyuddin, Mahesh Choolanib, Abdur Rahmana Lab-on-a-chip technology: impacting non-invasive prenatal diagnostics (NIPD) through miniaturisation, Lab Chip, 2014, 14, 841–854 Chorion villus biopsy (CVS) • is a prenatal test that involves taking a sample of tissue from the placenta • is usually performed between 11 and 13 weeks of gestation under ultrasound guidance. • carries around a 2% additional risk of causing a miscarriage. There are two types of CVS procedures: • Transcervical - in this procedure, a catheter is inserted through the cervix into the placenta to obtain the tissue sample (A). • Transabdominal - in this procedure, a needle is inserted through the abdomen and uterus into the placenta to obtain the tissue sample (B). A B The chorion is the outermost of the fetal membranes, and sampling instrument should not penetrate the amniotic cavity. Once removed, material needs expert dissection under microscope to pick fetal material free of contaminating maternal tissue. Prenatal diagnosis https://study.com/academy/lesson Prenatal diagnosis Chorionic villi are derived from the trophoblast, the extraembryonic part of the blastocyst. https://study.com/academy/lesson Prenatal diagnosis Chorionic villi can be used for • DNAextraction for molecular diagnostics For DNAtesting, results should always be compared to a control sample of the mother´s blood DNA, to ensure that the test result reflects the fetal genotype. • Rapid cytogenetic analysis of dividing cells already present. Such short-term cultures need to be confirmed with long-term cultures. Mosaicism detected in villi is difficult to interpret: retrospectively it often turns out to have been confined to the placenta Electrophoretogram of the quantitative fluorescent polymerase chain reaction (QF-PCR) products of maternal, paternal, and chorionic samples, tested using the amelogenin X/Y (AMXY) and D21S1414 (STR) markers. Note, in the chorionic biopsy the maternal X and the paternal chromosome Y marker. The paternal chromosome 21 marker is also present in chorionic sample. ps://doi.org/10.1016/B978-0-12-802971-8.00024-9 Amniocentesis(AMC) • is a prenatal test that involves taking a sample of amniotic fluid • amniotic fluid consists mainly of fetal urine and waschings from the lungs. • is usually performed between 14 and 20 weeks of gestation under ultrasound guidance. • carries around a 0,5 – 1,0 % additional risk of causing a miscarriage. Prenatal diagnosis It can be analyzed biochemically, or fetal cells can be isolated from fluid and cultured for cytogenetic analysis or fetal DNAcan be isolated from fluid for molecular analysis https://www.tabers.com/tabersonline/view/Tabers-Dictionary/756306/all/amniocentesis Amniocentesis(AMC) • is a prenatal test that involves taking a sample of amniotic fluid • amniotic fluid consists mainly of fetal urine and waschings from the lungs. • is usually performed between 14 and 20 weeks of gestation under ultrasound guidance. • carries around a 0,5 – 1,0 % additional risk of causing a miscarriage. Prenatal diagnosis It can be analyzed biochemically, or fetal cells can be isolated from fluid and cultured for cytogenetic analysis or fetal DNAcan be isolated from fluid for molecular analysis Biochemical analyses include testing for AFP, a protein produced by the fetal liver: a high level indicates that fetus has open lesion, most likely an open neural tube defect, but possibly an abdominal wall defect. https://www.tabers.com/tabersonline/view/Tabers-Dictionary/756306/all/amniocentesis Amniocentesis(AMC) • is a prenatal test that involves taking a sample of amniotic fluid • amniotic fluid consists mainly of fetal urine and waschings from the lungs. • is usually performed between 14 and 20 weeks of gestation under ultrasound guidance. • carries around a 0,5 – 1,0 % additional risk of causing a miscarriage. Prenatal diagnosis It can be analyzed biochemically, or fetal cells can be isolated from fluid and cultured for cytogenetic analysis or fetal DNAcan be isolated from fluid for molecular analysis Culture of cells from amniotic fluid for cytogenetic analysis to detect specific chromosomal abnormalities, takes around 2 weeks to obtain quality preparations. Newer technique that does not require cell culture is QF-PCR and array-CGH. https://www.tabers.com/tabersonline/view/Tabers-Dictionary/756306/all/amniocentesis Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers Is widely used as a rapid prenatal test for the common chromosomal trisomies Autosomal chromosome aneuploid pregnancies that survive to term, namely, trisomies 13, 18, and 21, X and account for 90% of chromosome abnormalities with a severe phenotype identified in prenatal samples. They are traditionally detected by full karyotype analysis of cultured cells. The average reporting time for a prenatal karyotype analysis is approximately 14 days, and in recent years, there has been increasing demand for more rapid prenatal results with respect to the common chromosome aneuploidies, to relieve maternal anxiety and facilitate options in pregnancy. The rapid tests that have been developed negate the requirement for cultured cells, instead directly testing cells from the amniotic fluid or chorionic villus sample, with the aim of generating results within 24 h of sample receipt. A quantitative fluorescence (QF)-PCR-based approach is now widely used and reported as a clinical diagnostic service. It may be used as a stand-alone test or as an adjunct test to full karyotype or array CGH analysis, which scan for other chromosome abnormalities not detected by the QF-PCR assay. Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers QF-PCR uses fluorescent labelled primers to amplify STR regions from DNA, by PCR. Short tandem repeats (STR, microsatelite) are highly polymorphic sequences found in the human DNA. https://cz.pinterest.com/pin/175921929169766990/ The amount of fluorescently labelled amplicons are measured after fragment length separation in capillary electrophoresis. QF-PCR is a quantitative method that determines the presence of different alleles which means the determination of chromosomal copy number It depends on using a gene analyzer to compare the relative amounts of product from multiplexed series of microsatelite markers from chromosomes 13, 18, 21, X and Y. Typically, seven loci from each chromosome would be amplified. Primers are designed and labeled so that the PCR products from each locus are clearly identifiable by their size and color. Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers Because microsatelite alleles vary slightly in length, different alleles of the same microsatelite often give peak at slihtly different position. Thus a locus may amplify as • two peaks (2 alleles with with different number of repeats – different length, heterozygous status) or • one larger peak (2 alleles with with the same number of repeats – the same length, homozygous status) If there is a trisomy the three alleles of each locus on that chromosome may • give three small peaks, or • two peaks in a 2:1 size ratio or sometimes a single large peak – an uninformative result for that locus Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers Typical electrophoretogram (Mix 1) showing the profile of a trisomic sample (47,XY, +21) QF PCR Work flow 1. DNAextraction from e.g. amniotic fluid 2. PCR amplification 3. Capillary electroforesis 4. Result analysis, diagnosis Prenatal diagnosis QF-PCR Quantitative PCR with fluorescence-labeled primers Prenatal diagnosis Non- Invasive Prenatal Testing (NIPT) Analysis of cell-free fetal DNA(cffDNA) in maternal blood Many researchers have attempted to develop noninvasive prenatal testing (NIPT) methods in order to investigate the genetic status of the fetus. The aim is to avoid invasive procedures such as chorionic villus and amniotic fluid sampling, which result in a significant risk for pregnancy loss. The discovery of cell-free fetal DNA circulating in the maternal blood has great potential for the development of NIPT methodologies. Methodologies developed are mainly based on counting DNAsequences via next-generation sequencing high resolution real-time PCR and microarray-based methodologies. Prof. Dennis Lo Yuk-ming, Li Ka Shing Professor of Medicine and Chairman of the Department of Chemical Pathology at The Chinese University of Hong Kong (CUHK) The discovery of cell-free fetal DNA(cffDNA) in maternal blood in 1997 provides the possibility to develop noninvasive prenatal testing, which can avoid the procedure associated fetal loss as well as the restriction of sampling time https://www.aacc.org/community/merit-awards/hall-of-fame/bios/t-to-z/yuk-ming Cell-free fetal DNA-based (cffDNA) • comprises small fragments of fetal DNA, thought to originate from trophoblast • cffDNA circulate in maternal plasma and form approximately 10% of the DNAfragments in maternal plasma • it is present in reliably measurable levels NIPT from 10 weeks of gestation and is cleared quickly from the maternal circulation hours after delivery, making it specific to that pregnancy. https://doi.org/10.1111/tog.12388 Non-Invasive Prenatal Testing (NIPS) NIPS - A • chromosomal aneuploidy detection NIPS - M • fetal RhD blood group genotyping • fetal sex determination for sex-linked disorders • diagnosis of monogenic diseases https://doi.org/10.1073/pnas.1617112113 NIPT The ability to identify fetal genetical anomalies has been possible since 2011 with the introduction of massively parallel sequencing (MPS) for this purpose. In 2011, this culminated in the clinical introduction of NIPS – A for aneuploidy using cfDNA. Subsequently, with higher depth of sequencing and improved bioinformatics analyses, NIPS expanded to include detection of a number of microdeletions. Genome-wide screening for copy number variants has also been reported and is now offered clinically. Noninvasive identification of fetal single-gene disorders, and ultimately analysis of the fetal genome, has become the “next frontier” in prenatal diagnosis. NIPS - A In aneuploidy, DNAfrom each chromosome is quantified and common autosomal trisomies are detected based on a difference in the proportion of each chromosome (e.g., chromosome 21 compared to the other chromosomes from that fetus). Following complex biostatistical analysis, a result of ‘low risk’ or ‘high risk’ is given. MPS technology has continued to advance and two different subtypes are now recognised: (a) massively parallel shotgun sequencing, whereby the whole genome is randomly sequenced, (b) ‘targeted’ MPS in which only specific genomic regions known to contain the chromosome (or single nucleotide polymorphism [SNP]) of interest are sequenced and compared to reference regions. https://doi.org/10.1186/s13039-019-0441-5 Molecular genetic testing Direct testing detects the specific disease-causing pathogenic variants or foreign DNAsequence Indirect testing (gene tracking) This type of testing is commonly referred to as linkage analysis. Polymorphic markers closely associated with the disease-causing gene are used to assess whether an individual has inherited the pathogenic allele of the disease-causing gene responsible for the disease phenotype. Linkage analysis is based on tracking the inheritance of polymorphic markers in a family with a genetic disease. If the markers and the disease-associated gene are in proximity, then the likelihood of a recombination event occurring between them is minimal. Thus, coinheritance of the markers and the disease-associated gene is likely. The advantage of linkage analysis is that the gene of interest need only be mapped to a chromosomal location. Limitations to this technology include significant labor and turnaround-times, the need to analyze samples from many family members, and the possibility of having to use numerous markers to obtain informative data. Can be used a direct or indirect analysis Direct testing provides evidence of a pathological variant responsible for producing the illness. It is determined whether the sequence of the DNA(nucleotide sequence) has changed. These assays require that pathological variant and/or the gene sequence of interest is known. Sequence changes testing methods can be divided into two groups: 1. Scoring – methods for detecting specific sequence changes 2. Scanning – methods for scannig a gene for any sequence change scoring scanning Scoring - methods for detecting specific sequence changes Searching for known sequence change is possible for: • The disease in question may always be caused by exactly the same sequence change An example is Achondroplasia Achondroplasia arise from a change in the same base pair of FGFR3, that are autosomal dominant around 98% of persons with achondroplasia have a c.1138G>A gene change, and 1% have a c.1138G>C mutation targeted mutation analysis is the routinely employed molecular test is the most common of the skeletal dysplasias that result in marked short stature (dwarfism) method of genotyping by melting point analysis on High Resolution Melting (HRM) on the LightCycler® 480 System platform using the LightSNiP assay. Scoring - methods for detecting specific sequence changes Searching for known sequence change is possible for: • The disease in question may always be caused by exactly the same sequence change An example is Achondroplasia • A disease may be caused by various different sequence changes, but one or a few variants may be so frequent in a particular population that it is worth first checking for these befor going on to a more general search. An example is Cystic Fibrosis; over 2000 different variants have been reported, but 65% of all pathogenic variants of CFTR gene in Europeans are one particular deletion of 3 nucleotides p. F508del Cystic fibrosis In people with CF, patogenic variants in the cystic fibrosis transmembrane conductance regulator (CFTR) gene cause the CFTR protein to become dysfunctional. When the protein is not working correctly, it’s unable to help move chloride -- a component of salt -- to the cell surface. Without the chloride to attract water to the cell surface, the mucus in various organs becomes thick and sticky. The airways fill with thick, sticky mucus, making it difficult to breathe. The thick mucus is also an ideal breeding ground for bacteria and fungi. Cystic fibrosis Most genetic tests only screen for the most common CF mutations: Allele-specific polymerase chain reaction Allele-specific polymerase chain reaction (AS-PCR) is a technique based on allele-specific primers, which can be used to analyze single nucleotide polymorphism. The allele-specific PCR is also called the (amplification refractory mutation system) ARMS-PCR corresponding to the use of two different primers for two different alleles. One is the mutant set of primers which are refractory (resistant) to the normal PCR, and the other is the normal set of primers, which are refractory to the mutant PCR reaction. The 3’ ends of these primers are modified such that one set of the primer can amplify the normal allele while others amplify the mutant allele. This mismatch allows the primer to amplify a single allele. Cystic fibrosis Although over 2000 different variants in the CFTR gene have been described in cystic fi most of these have been seen in only one or a very few cases. A small number of patologiocal variants are relatively common. Mutation testing in cystic fibrosis therefore starts by checking for these common mutati WT - F508del (+STR) MT + WT pro F508del (+STR) Elucigene® CF-EU 2v1 typical electropherogram obtained through ARMS analysis Scoring - methods for detecting specific sequence changes Searching for known sequence change is possible for: • The disease in question may always be caused by exactly the same sequence change An example is Achondroplasia • A disease may be caused by various different sequence changes, but one or a few variants may be so frequent in a particular population that it is worth first checking for these befor going on to a more general search. An example is Cystic Fibrosis; over 2000 different variants have been reported, but 65% of all pathogenic variants of CFTR gene in Europeans are one particular deletion of 3 nucleotides p. F508del • The test may be to check somebody for a family pathogenic variant that has already been identified and characterized in other family members • The test may be to check samples from haelthy controls to make sure a variant found in a patients is not a non-pathogenic variant present in normal population Scanning- methods for scanning a gene for any sequence changes A dignostic laboratory often needs to check every exon of candidate gene in a patient to look for patogenic variants. Given the average sizes of exons and introns (145 bp and 3365 bp, respectively) this usually means PCR amplifying and sequencing each exon individually. Various methods were developed to save sequencing costs by scanning each exon quickly and cheaply to eliminate those that apparently contained no variants (SSCP, DGGE, dHPLC). The cost of sequencing has now fallen to the point that this approach is seldom used, except for scanning a gene to check for deletions or duplications of whole exon An example Duchenne muscular dystrophy (DMD) Duchenne muscular dystrophy (DMD) a genetic disorder characterized by progressive muscle degeneration and weakness due to the alterations DMD occurs because the mutated DMD gene fails to produce any functional protein called dystrophin that helps keep muscle cells intact. The other dystrophinopathy is Becker muscular dystrophy (BMD, a mild form of DMD) Individuals with BMD genetic mutations make dystrophin that is partially functional, which protects their muscles from degenerating as badly or as quickly as in DMD. Muscles are made up of bundles of fibers (cells). A group of interdependent proteins along the membrane surrounding each fiber helps to keep muscle cells working properly. When one of these proteins, dystrophin, is absent, the result is Duchenne muscular dystrophy (DMD); poor or inadequate dystrophin results in Becker muscular dystrophy (BMD). Duchenne muscular dystrophy (DMD) has an X-linked recessive inheritance pattern and is passed on by the mother, who is referred to as a carrier. The dystrophin gene is the largest gene yet identified in humans and is located in the short arm of the X chromosome, in the Xp21.2 locus (a locus is the position of a gene on a chromosome). The majority (60 - 70 %) of mutations of the dystrophin gene are deletions of one or more complete exons. These deletions are relatively easy to detect in an affected male. Duchenne muscular dystrophy (DMD) 4 sets multiplex PCR Tube 1 Pm 535 pb exon 3 410 pb exon 43 357 pb exon 13 238 pb exon 6 207 pb Tube 2 exon 49 439 pb exon 50 271 pb exon 47 181 pb exon 60 139 pb exon 52 113 pb Tube 3 exon 19 459 pb exon 8 360 pb exon 4 196 pb Tube 4 exon 48 506 pb exon 44 426 pb exon 51 388 pb exon 45 307 pb exon 53 212 pb exon 42 155 pb confirmed DMD: deletion DMD exons 45, 47, 48 P m 3 43 13 6 49 50 47 60 52 19 8 4 48 44 51 45 53 42 To check for partial deletions,individual exons ofthe gene are amplified by PCR. Primers are designed to match sequences in the introns flanking an exon, so that the product contains the complete exon and some intronic sequence. Each exon gives a different sized productby varying the amountof intron included. A series of PCR reactions can be performed in one operation (multiplexed). The mix of products from all PCR amplifications is run on an electroforetic gel. Duchenne muscular dystrophy (DMD) Carrier testing in women is more difficult than testing a boy because a carrier would be hetorozygous and every exons of the dystrophin gene would amplify from her normal chromosome. A quantitative test is required - MLPA Duchenne muscular dystrophy (DMD) Multiplex ligation-dependent probe amplification (MLPA) is a variation of the multiplex PCR that permits amplification of multiple targets with only a single primer pair. It detects copy number changes at the molecular level, and software programs are used for analysis. MLPA consists of the following steps: 1.Denaturation 2.Hybridization 3.Ligation 4.Amplification (by PCR) 5.Fragment Separation and Data Analysis 1 - Denaturation and 2 – Hybridization Denaturation involves separation of the annealed DNAstrands, so that double-stranded DNA becomes single-stranded. Hybridization involves hybridizing the DNA sample to specific probes. Because it is a multiplex technique, you can analyze each sample by up to 60 probes simultaneously, thus targeting different sites! These probes have a primer sequence that binds to the PCR-primer in the amplification process. All different probes will have the same primer binding sequence. Additionally, the probes also have a hybridization sequence complementary to the target site that will allow the probe to bind to the DNA. Both probes will hybridize on adjacent sites on the DNAstrand. One of the probes from the pair contains a stuffer sequence, which is different in length for each target site. The length of the stuffer sequence changes between different probes, allowing multiplexing. So, you can expect each amplification product to have a unique length! 3-Ligation The ligation step will bind the two probes together. In this step, a specific enzyme called DNAligase is used. It binds the probes that are already hybridized on adjacent sites of the DNA strand at the target site. The ligase used in MLPA protocols is ligase-65, an NAD-dependent ligase enzyme. Both probes contain the binding sites for PCR-primers. This means, if we were to use the probes as a single molecule, we would obtain an amplification product, even without the DNAtarget site, thus giving us non-specific amplification. The enzyme ligase is extremely specific: if there are any mismatches between the probe and the target site, the ligase will not be able to bind the probes and no amplification would occur. Consequently, MLPA detects specific point mutations, and even distinguishes between pseudogenes and the real target gene. 4-Amplification The next step is amplification, which is essentially a polymerase-chain reaction (PCR). For the PCR step, a polymerase, dNTPs, and a forward and reverse primer are added. Since all of the probes have the same PCR-primer sequence, it will only be necessary to add one pair of universal primers to study all of our targets. The forward primer is fluorescently labelled, allowing visualization and quantitation during analysis. 5-Fragment Separation and Data Analysis After amplification, the fragments are separated by capillary electrophoresis. Capillary electrophoresis separates fragments based on their length, and shows different length fragments as peak patterns, called an electropherogram. Each amplicon has a different known size, due to the stuffer sequence on each specific probe, and therefore each amplicon can be quantified during data analysis. The data obtained by capillary electrophoresis will be the input for the analysis. MRC- Holland provides a free software for data analysis – Coffalyser. By comparing each sample to a set of reference samples, we can obtain a probe ratio. This probe ratio will inform us of how many copy numbers a gene has. Since most human genes are diploid, if the sample presents two copies, the ratio will be 1.0; i.e. the sample probes have obtained the same number of genes as the reference sample. However, if the ratio is 0.5 there was only one copy of the gene in the individual, which probably means a heterozygous deletion of the target gene. If, on the other hand, the ratio is 1.5, there is, probably, a heterozygous duplication of a gene. MRC-Holland offers many different kits that may have the solution for your problems. DNA sequencing is the process of determining the sequence of nucleotide bases For almost all of past 30 years all DNA sequencing has been based on a single basic technic, dideoxy or Sanger sequencing. DNA sequencing is the process of determining the sequence of nucleotide bases Sanger sequencing are performed in an automated fashionvia sequencingmachine. Each method follows three basic steps. 1. DNA Sequence For Chain Termination PCR The DNA sequence of interest is used as a template for a special type of PCR called chain-terminationPCR. Chain-terminationPCR works just like standard PCR, but with one major difference: the addition of modified nucleotides (dNTPs) called dideoxyribonucleotides (ddNTPs). In the extensionstep of standard PCR, DNA polymerase adds dNTPs to a growing DNA strand by catalyzing the formation of a phosphodiester bond betweenthe free 3’-OH group of thelast nucleotideand the5’-phosphateof the next. In chain-termination PCR, the user mixes a low ratio of chain-terminating ddNTPs in with the normal dNTPs in the PCR reaction. ddNTPs lack the 3'-OH group required for phosphodiester bond formation; therefore,when DNA polymerase incorporates a ddNTP at random, extension ceases. The result of chain-terminationPCR is millions to billions of oligonucleotidecopies of the DNA sequence of interest, terminatedat a random lengths (n) by 5’-ddNTPs. In automated Sanger sequencing, all ddNTPs are mixed in a single reaction, and each of thefour dNTPs has a unique fluorescentlabel. 2. Size Separation by Gel Electrophoresis In the second step, thechain-terminatedoligonucleotides are separatedby size via gel electrophoresis. In gel electrophoresis, DNA samples are loaded into one endof a gel matrix, and an electric current is applied; DNA is negatively charged, so theoligonucleotides will be pulled toward the positive electrodeon the opposite side of thegel. Because all DNA fragments have the same chargeper unit of mass, the speed at which theoligonucleotides move will be determined only by size. The smaller a fragment is, the less friction it will experience as it moves through thegel, andthe faster it will move. In result, the oligonucleotides will be arranged from smallest to largest, reading thegel from bottom to top. In automated Sanger sequencing, all oligonucleotides are run in a single capillary gel electrophoresis within the sequencingmachine. 3. Gel Analysis & Determination of DNA Sequence The last step simply involves reading the gel to determine the sequenceof the input DNA. BecauseDNA polymerase only synthesizes DNA in the 5’ to 3’ direction starting at a provided primer, each terminal ddNTP will correspond to a specific nucleotidein the original sequence (e.g., the shortest fragment must terminateat the first nucleotide from the 5’ end, the second-shortestfragmentmust terminate at thesecondnucleotidefrom the 5’ end, etc.) Therefore, by reading thegel bands from smallest to largest, we can determine the 5’ to 3’ sequence of theoriginal DNA strand. In automated Sanger sequencing, a computer reads eachbandof the capillary gel, in order, using fluorescence to call the identity of eachterminal ddNTP. In short, a laser excites the fluorescent tags in eachband, anda computer detects the resultinglight emitted.Because eachof the four ddNTPs is taggedwith a different fluorescent label, the light emitted can be directly tied to the identity of theterminal ddNTP. The output is called a chromatogram, which shows thefluorescent peak of eachnucleotidealongthe length of the template DNA. DNA sequencing is the process of determining the sequence of nucleotide bases Several revolutionary new sequencing technologies have burst onto the scene. Collectively called „next generation sequencing“ or „massively parallel sequencing Development of new sequencing methods allowed faster and more economical genomic research. With these technologies, it is now possible to determine the complete sequence of human genome in a short time period and at a relatively low cost. https://www.biochain.com/gener al/from-sanger-to-next-generation-sequencing/ DNA sequencing Gupta N., Verma V.K. (2019) Next-Generation Sequencing and Its Application: Empowering in Public Health Beyond Reality. In: Arora P. (eds) Microbial Technology for the Welfare of Society. Microorganisms for Sustainability, vol 17. Springer, Singapore. https://doi.org/10.1007/978-981-13-8844-6_15 DNA sequencing Basic features and performances of NGS platforms. DNA sequencing Traditional Sanger sequencing compared with next-generation sequencing technology. In each method, dyed,unextendable bases are utilized to create a fluorescent signal that can be translated into a sequence of nucleotides. Subtle differences in the two methods lead to vast differences in throughput. This image was reproduced from figure 1 in Muzzey, Evans, and Lieber (2015). It is licensed under Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/). Next generation sequencing“ or „massively parallel sequencing NGS has the potential to find causal mutations, including de novo, novel and familial mutations, associated with genetic diseases and, due the variable phenotypic presentations of the disorder, vastly improve molecular diagnosis. First generation DNAsequencing with chain-terminating inhibitors invented by Sanger in 1977, led to many genetic discoveries and has been widely used for over 30 years in research and diagnostic laboratories. Although considered a major technological breakthrough, and still finding utility today for variant verification, the technique has limitations, in particular when examining large regions of the genome. More recently NGS has begun to replace Sanger sequencing due its ability to sequence large numbers of genes, the whole exome (protein-coding regions) or entire genome at once. Thus applications of NGS include targeted gene panels, whole exome sequencing (WES) and whole genome sequencing (WGS). Custom gene panel testing allows for screening of multiple potentially clinically relevant genes and for more flexibility in phenotype–genotype correlations than required when testing individual genes. WES focusses on the protein coding regions in the genome, comprising approximately 1–2% of the genome, attributable to ~85% of disease related mutations. In contrast, WGS provides information on the entire genome (both coding and non-coding regions), providing additional information on mutations in regulatory regions, as well as copy number variations with higher efficiency than WES. The ~99% of the genome not included as exome sequence also contains untranslated regions which may have a regulatory role (e.g., non-coding RNAs or transcription binding sites) along with potential protein coding sites yet to be annotated as genes The impact of variants found in non-coding regions are not currently well understood, however it is feasible that a single or a combination of variants could have a significant impact on the pathology. This is most evident for non-coding variants that may influence expression levels or mRNA splicing, affecting protein abundance or isoforms. Lékařská fakulta Masarykovy univerzity 2021