Genetic analysis of individual genomes and single cells; Genome-wide association studies (GWAS) Flashcards
Whole-genome sequencing (WGS) has become relatively cheap, is quick and reliable for accurately sequencing individual genomes.
Personal genomics is increasingly utilised by clinicians and hospitals for
WGS and identification of genetic disorders like anorexia, Alzheimers and autism.
Whole-genome sequencing (WGS) has led to
improved treatment of diseases, based on the individual genome
Whole-genome sequencing (WGS)
Example: ARVD/C is a rare heart disease that leads to irregular electrical impulses that can be lethal.
Native Newfoundlanders have a very high incidence ARVD/C.
Through individual genome sequencing, a mutation in the AVRD5 gene has been identified as the cause of such cases of premature death (approximately 50% of males and 5% of females die by age 40, and 80% of males and 20% of females die by age 50).
Individuals carrying this mutation are now being implanted with internal cardiac defibrillators that can restart their hearts if electrical impulses stop or become irregular.
Whole exome sequencing (WES) is similarly used in clinical settings identify genetic disorders and ultimately to the treatment of these.
Example: Nicholas Volmer
– intestinal fistulas.
>100 surgeries by age 3.
WES performed and a mutation in X-linked inhibitor of apoptosis (XIAP) gene identified.
Led doctors to perform a bone marrow transplant that saved his life.
1st kid whose life has been saved by sequencing!
The NIH started the “Undiagnosed Diseases Network” with the goal to
use WGS and WES to diagnose rare and mysterious disease conditions of unknown genetic basis.
“Undiagnosed Diseases Network”
Exome sequences from an individual with a clinical disorder are compared to exome sequences from healthy family members and reference sequences - to identify mutations that may be involved in the disease. The program has already diagnosed over 40 cases.
It is now possible to sequence the genome from a single cell!
Single-cell sequencing (SCS)
Single-cell sequencing (SCS)
involves isolating genomic DNA from a single cell, then subjected to whole-genome amplification (WGA) using PCR - to produce sufficient DNA to be sequenced.
Amplification of the genome to produce enough DNA for sequencing without introducing errors remains a major challenge that researchers are working on so that SCS can become a more reliable and accurate technique for genetic testing.
WGA without introducing errors remains a major challenge – high-fidelity polymerases.
SCS is valuable for analysing:
- Somatic cell mutations,
i.e. mutations that arise in somatic cells such as in a skin cancer, which are not heritable. - Germ-line mutations,
i.e. heritable mutations that are transmitted to offspring via gametes. - Genetic variations from cell to cell,
e.g. cancer cells from a tumor often show genetic diversity. Understanding variations in genetic diversity and gene expression by individual cells within a tumor could lead to better and more specific treatment options.
Sequencing genomes from individual egg or sperm cells, especially for couples undergoing in vitro fertilisation, can identify
carrier conditions or specific germ-line mutations that could result in a genetic disorder in the offspring
Single-cell sequencing (SCS)
Now possible to isolate and sequence both DNA and RNA from single cells – the same cell!
Enables the
comparison of the genes present in a single cell and their relative expression levels for each transcript encoded by that cellular genome.
Single-cell RNA sequencing (scRNA-seq)
scRNA-seq can be done non-destructively (Live-seq).
Use PCR to amplify genomic DNA (for sequencing).
mRNA is reverse transcribed into cDNA and cloned in a library and sequenced.
scRNA-seq provides:
A quantitative transcriptome analysis in which the relative levels of RNA expressed in a cell can be determined.
Similar to gene-expression microarray analysis, but does not need prior sequence information – more comprehensive.
Dataplot of 325 ILCs from mouse marrow cells - groups ILCs into similar clusters based on shared gene-expression patterns. Each dot represents an individual cell, plotted against its expression levels for all genes analyzed by RNA-seq.
scRNA-seq of mouse bone marrow progenitor cells enabled identification of different subsets of ILCs by their RNA-expression patterns. Such analysis reveals similarities in gene expression but significant differences in the transcriptomes of ILCs that, by phenotype, might appear to be the same. For example, in the figure, note how the RNA-seq profiles of RNAs expressed by cells in cluster C10 are very different than the profiles of RNAs expressed by cells in cluster C3.
Heatmap – displays RNA expression levels for selected genes in cell clusters. Columns represent scRNA-seq for each of the 325 cells, and each row shows the expression level heat map for a specific gene. b-actin mRNA is control (bottom row).
Shown here is a Manhattan plot from a GWAS for Type 2 diabetes. The study revealed 386,371 genetic markers, clustered by chromosome number (x-axis). Markers above the black line (y-axis) appeared to be significantly associated with the disease.
These genes can therefore be causally linked to the potential of individuals carrying mutations (e.g. SNPs) to be at a higher predisposition to contract Type 2 diabetes.
