Principles of Human Genetics Part 31 More discrete sequence alterations rely heavily on the use of the PCR, which allows rapid gene amplification and analysis.. Moreover, PCR makes it
Trang 1Chapter 062 Principles of
Human Genetics
(Part 31)
More discrete sequence alterations rely heavily on the use of the PCR, which allows rapid gene amplification and analysis Moreover, PCR makes it possible to perform genetic testing and mutational analysis with small amounts of DNA extracted from leukocytes or even from single cells, buccal cells, or hair roots Screening for point mutations can be performed by numerous methods (Table 62-9); most are based on the recognition of mismatches between nucleic acid duplexes, electrophoretic separation of single- or double-stranded DNA, or sequencing of DNA fragments amplified by PCR DNA sequencing can be performed directly on PCR products or on fragments cloned into plasmid vectors amplified in bacterial host cells
Trang 2RT-PCR may be useful to detect absent or reduced levels of mRNA expression due to a mutated allele Protein truncation tests (PTT) can be used to detect the broad array of mutations that result in premature termination of a polypeptide during its synthesis The isolated cDNA is transcribed and translated
in vitro, and the proteins are analyzed by gel electrophoresis Comparison of electrophoretic mobility with the wild-type protein allows detection of truncated mutants
The majority of traditional diagnostic methods are gel-based Novel technologies for the analysis of mutations, genotyping, large-scale sequencing, and mRNA expression profiles are in rapid development DNA chip technologies allow hybridization of DNA or RNA to hundreds of thousands of probes simultaneously Microarrays are being used clinically for mutational analysis of several human disease genes, as well as for the identification of viral sequence variations Together with the knowledge gained from the HGP, these technologies provide the foundation to expand from a focus on single genes to analyses at the scale of the genome Faster and cheaper sequencing technologies are under development, and it has been anticipated that sequencing the whole genome of an individual for a cost of ≤$1000 will become a reality within this decade The availability of comprehensive individual sequence information is expected to have
a significant impact on medical care and preventative strategies, but it also raises
Trang 3ethical and legal concerns how such information may be used by insurers and employers
A general algorithm for the approach to mutational analysis is outlined in Fig 62-14 The importance of a detailed clinical phenotype cannot be overemphasized This is the step where one should also consider the possibility of genetic heterogeneity and phenocopies If obvious candidate genes are suggested
by the phenotype, they can be analyzed directly After identification of a mutation,
it is essential to demonstrate that it segregates with the phenotype The functional characterization of novel mutations is labor intensive and may require analyses in vitro or in transgenic models in order to document the relevance of the genetic alteration
Prenatal diagnosis of numerous genetic diseases in instances with a high
risk for certain disorders is now possible by direct DNA analysis Amniocentesis
involves the removal of a small amount of amniotic fluid, usually at 16 weeks of gestation Cells can be collected and submitted for karyotype analyses, FISH, and mutational analysis of selected genes The main indications for amniocentesis include advanced maternal age above age 35, abnormal serum triple marker test (α-fetoprotein, βhuman chorionic gonadotropin, pregnancy-associated plasma protein A, or unconjugated estriol), a family history of chromosomal abnormalities, or a Mendelian disorder amenable to genetic testing Prenatal
diagnosis can also be performed by chorionic villus sampling (CVS), in which a
Trang 4small amount of the chorion is removed by a transcervical or transabdominal biopsy Chromosomes and DNA obtained from these cells can be submitted for cytogenetic and mutational analyses CVS can be performed earlier in gestation (weeks 9–12) than amniocentesis, an aspect that may be of relevance when termination of pregnancy is a consideration Later in pregnancy, beginning at about 18 weeks of gestation, percutaneous umbilical blood sampling (PUBS) permits collection of fetal blood for lymphocyte culture and analysis In combination with in vitro fertilization (IVF) techniques, it is even possible to perform genetic diagnoses in a single cell removed from the four- to eight-cell embryo or to analyze the first polar body from an oocyte Preconceptual diagnosis thereby avoids therapeutic abortions but is extremely costly and labor intensive Lastly, it has to be emphasized that excluding a specific disorder by any of these approaches is never equivalent to the assurance of having a normal child
Mutations in certain cancer susceptibility genes, such as BRCA1 and
BRCA2, may identify individuals with an increased risk for the development of
malignancies and result in risk-reducing interventions The detection of mutations
is an important diagnostic and prognostic tool in leukemias and lymphomas The demonstration of the presence or absence of mutations and polymorphisms is also relevant for the rapidly evolving field of pharmacogenomics, including the identification of differences in drug treatment response or metabolism as a function of genetic background For example, the thiopurine drugs
Trang 56-mercaptopurine and azathioprine are commonly used cytotoxic and immunosuppressive agents They are metabolized by thiopurine methyltransferase (TPMT), an enzyme with variable activity associated with genetic polymorphisms
in 10% of Caucasians and complete deficiency in about 1/300 individuals Patients with intermediate or deficient TPMT activity are at risk for excessive toxicity, including fatal myelosuppression Characterization of these polymorphisms allows mercaptopurine doses to be modified based on TPMT genotype Pharmacogenomics may increasingly permit individualized drug therapy, improve drug effectiveness, reduce adverse side effects, and provide cost-effective pharmaceutical care
Further Readings
Altshuler D et al: for The International HapMap Consortium: A haplotype map of the human genome Nature 437:1299, 2005
Guttmacher AE, Collins FS: Realizing the promise of genomics in biomedical research JAMA 294:1399, 2005 [PMID: 16174701]
——— et al: The family history—more important than ever N Engl J Med 351:2333, 2004
Trang 6Rockman MV, Kruglyak L: Genetics of global gene expression Nat Rev Genet 7:862, 2006 [PMID: 17047685]
Roden DM et al: Pharmacogenomics: Challenges and opportunities Ann Intern Med 145:749, 2006 [PMID: 17116919]
Service RF: Gene sequencing The race for the $1000 genome Science 311:1544, 2006 [PMID: 16543431]
Wolfsberg TG et al: A user's guide to the human genome Nat Genet 35(Suppl 1): 2003
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