Molecular genetics and cytogenetics
laboratory and methods
KARLA PLEVOVÁ
21.2.2023
Statement
This presentation is intended exclusively for educational purposes.
Every form of misuse, including copying, distribution and sharing on public online
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Outline of the presentation
What to expect from a molecular genetics and cytogenetics laboratory (MGC lab)?
How does it look in the MGC lab?
What methods are available in the MGC lab?
What to expect from a MGC lab?
MGC LAB = PARTNER
Specifics of a MG lab – a need for assays designed for individual families or individual patients
→ a high proportion of laboratory developed tests compared to other diagnostic labs in hospitals
Discuss with the staff, learn what methods they use, know what the methods can be good for
Application of results
Establishing and refining diagnosis
Prenatal and preimplantation testing
Hereditary predisposition assessment
Disease prognostication
Treatment optimization
Disease activity monitoring
Disease complication diagnostics
Prochazkova et al, BMC
Medical Education 2019
Technical aspects of the laboratory methods
Target regions, analytes
Specificity and sensitivity, limit of detection, …
Tools for data analysis and their limitations
Time for processing – few hours or few days?
Standardization and validation
Regular quality assessment
Compliance with legislation regulations
→ a basis for laboratory test request
→ expectations and outcomes
Laboratory manual!
Practical example
BRONCO diagnostic panel for hereditary cancer syndromes
• What genetic syndrome
am I looking for?
• Are suspect genes
included in the panel?
• What defects could I
expect?
• How quickly do I need the
result?
• …
• Is the method suitable for
answering my questions?
Result of a laboratory test
The report is an essential part of any laboratory test
Content – concise but comprehensive:
What exactly was tested
What method was used
What results were obtained
Who reports the results
Who reviewed the results
What preanalytic, analytic, and postanalytic factors could influence the results
What cannot be identified (e.g. failed or low covered regions)
Comply with ISO 15189 technical requirements for medical laboratories
How does it look the MG lab?
Sample
reception
Primary
processing
Pre-PCR
area
Post-PCR area
Other post-PCR
methods
Cultivation
room
Analytical
space
Pre-PCR Post-PCR
Sample biobank Computation, data storage
Quality control requirements
Internal QC
External QC
national
international
Needed for method (and laboratory) accreditation
Compliance with international regulations for in vitro diagnostic methods
https://ukneqas.org.uk/about-us/
Sample processing
and separation
Diverse input material
(peripheral blood, tissue
specimens etc.)
Sterile hoods (esp. in
connection with cell cultivation
and biobanking of samples)
Cell separation needed in
specific contexts (e.g. analysis
of somatic changes
Materials used
Peripheral blood
Bone marrow
Liquid biopsies
Aspirates
Fine-needle biopsies
Fresh tissue
Formalin-fixed paraffin-embedded (FFPE) tissue
Swabs (e.g. buccal)
Postnatal genetics
X
Prenatal testing
X
Oncology
Peripheral blood processing
Different cell population used according to the application:
Leukocytes
Mononuclear cells
Granulocytes
Lymphocytes
Specific cell subpopulations
Why to perform cell separation?
Example of TP53 gene testing in chronic lymphocytic leukemia
Polymerase chain reaction (PCR)
Fundamental reaction of molecular biology and genetics
Amplification of regions of interests
PCR assembling in pre-PCR area
Carried out in thermocycler
Various modifications
real-time PCR
Quantitative method – fluorescent detection
of generated products
Need for specific primers and probes
Relative and absolute quantification
test sample
Droplet digital PCR (ddPCR)
Alternative method for marker absolute quantification
Highly precise
Need for specific instrumentation
1
2
3
4
Next-generation sequencing (NGS)
~ massively parallel sequencing (MPS)
PCR amplification of DNA fragments or direct sequencing of individual fragments (single molecule
sequencing)
The most common approach – sequencing by synthesis (Illumina sequencers)
Millions of fragments are amplified simultaneously (vs capillary sequencer max 96 reactions)
Short reads (tens to hundreds base pairs)
NGS - targeted regions
Illumina machines and their capacity
HiSeq
4000
12 genomes/run,
1.5 TB/run
NextSeq
500
1 genome/run,
120 GB/run
MiSeq
0.15 genome/run,
15 GB/run
NovaSeq
48 genomes/run,
6 TB/run
MiniSeq
0.07 genome/run,
7.5 GB/run
iSeq
0.01 genome/rin,
1.2 GB/run
New sequencing machines on the market
Oxford Nanopore Technologies
Element Biosystems
Complete Genomics
Singular Genomics
PacBio
Short-read vs. long-read sequencing
Kraft & Kurth, Medizinische Genetik 2019
Schwarz et al, Medizinische Genetik 2021
NGS – regions of interest
genome exome selected genes or loci
3 200 000 000 bp
30 x read depth
20 000 genes
100 x read depth
< 100 genes
≥ 1000 x read depth
Practical example
Limit of detection (LoD) of various NGS methods
McNulty et al, J Mol Diagn 2020
In theory… (binomial sampling statistics)
method Amplicon Panel WES WGS
coverage 10 000 x 1000 x 100 x 30 x
LoD ~ 1 % ~ 5 % 15–20 % ~ 30 %
NGS – diverse targeted markers
BCR-
ABL
AGTAATATGCCT
ACCAATATAACT
AG-ACCATATG-CT
Panel NGS
Sets of selected regions of interest
Target enrichment by amplification
or hybridization
Why to use gene panels:
One disease can be associated with
variants in different genes
Certain gene is diagnostically relevant for
several diseases
Jennings et al, J Mol Diagn 2017
Practical example
LYNX panel
– diagnostics of molecular markers
in lymphoid malignancies
1CLL, 2MCL, 3FL, 4DLBCL, 5ALL, 6Ph-like ALL
Navrkalova et al, J Mol Diagn 2021
Whole exome sequencing (WES)
Identification of causative variants
Discovery of novel genetic markers
Searching for treatment targets
Whole genome sequencing (WGS)
Mainly experimental method for exploring unknown variants
Applications similar to WES, additional information about non-coding regions and chromosomal
abnormalities
Typical sequencing coverage ~ 30–100x – detection of somatic clonal or germline mutations
Shallow sequencing (~ 0.5-10x coverage) – genome-wide detection of chromosomal
abnormalities, low yield of mutation detection
In clinical practice a potential benefit of combination of shallow and panel sequencing
8
11
13
18
Practical example
Benefits of NGS in cancer diagnostics and monitoring
Reconstruction of clonal architecture and cancer evolution
Need for multidisciplinary team
– biologists, geneticists, computational scientists, bioinformaticians, statisticians
Single-cell technologies
Experimental methods
Applications in cancer research, immunology, developmental biology, …
Analysis of DNA variants, chromatin activity, RNA expression profiles, protein expression, …
Coexistence of cellular features in single cells
diagnosis
pretreatment (run1)
pretreatment (run2)
2nd relapse
3rd relapse
https://www.10xgenomics.com/
Cytogenomics lab
Sample
reception
Primary
processing
Pre-PCR
area
Post-PCR
area
Microscopic techniques
Cultivation
Analytical space
Sample biobank
Schoumans J et al, 2016
Aneu-
ploidy
CNA Poly-
ploidy
Clonal
heterogeneity
Focal
amplification
Balanced
rearrangements
Unbalanced
rearrangements
cn-LOH
Classical
cytogenetics
+++ + +++ +++ ++ +++ +++ Interphase
FISH +++ ++ + +++ +++ +++ ++ ArrayCGH
+++ ++ - + +++ - ++ -
CGH+SNP
array
+++ +++ + + +++ - ++ ++
SNP array +++ +++ ++ ++ +++ - ++ +++
CNA – copy number alteration, gains or lossess of genetic material
cn-LOH – copy neutral loss of heterozygozity
Cytogenomics methods
Comparison of sensitivity of the techniques
Classical cytogenetics
chromosome banding techniques
Methods not requiring PCR
Imaging methods
Cheap
Clonal composition assessment
Molecular cytogenetics
Fluorescent in situ hybridization (FISH)
Targets specific regions based on DNA sequence
Detection of chromosomal abnormalities with diagnostic, prognostic and predictive value
Probe types:
centromeric genewhole chromosome
Molecular cytogenetics
FISH methods for genome-wide analysis
mFISH mBAND
Genomic arrays
Molecular cytogenetic technique for detection of genomic gains and losses
Detection of copy-neutral loss of heterozygosity
Not possible to detect balanced rearrangements
Precise breakpoint localization, identification of affected genes
High resolution, genome-wide
Working with DNA, no need for viable cells
Equipment for genomic arrays
hybridization oven washing & staining system scanner
Affymetrix GeneChip System
Practical example
Muscular dystrophy
Panel NGS – imbalance of SNPs on chr2
Genomic array – UPD chr2 in 80% of cells – germline mosaicism
Take-home messages
• Discuss
• Standardize
• Integrate
The end…
Contact:
karla.plevova@mail.muni.cz or plevova.karla@fnbrno.cz
Thank you for your attention!