Genetics
Chromosome and gene aberrations
Chromosomal abnormalities
Structural
Numeric
Gene mutatios Rare alleles Polymorphisms
Gene mutation - types
Normal state DNA
ATGCAGGTGACCTCAGTG TACGTCCACTGGAGTCAC
Mutation „i
DNA
ATGCAG TGACCTCAGTG TACGTCG ACTGGAGTCAC
AUGCAGGUGACCUCAGU G
PROTEIN
Met-Gln-Val-Thr-Ser-Val
AUGCAG UGACCUCAGUG
PROTEIN
Met-Gln-Leu-Thr-Ser-Val
Examples-hemoglobin Sin sickle heterozygote advantage
Gene mutation - types
■ Normal state ■ Mutation „nonsense"
■ DNA ■ DNA
■ ATGCAGGTGACCTCAGTG ■ ATGCAGGTGACCTGAGTG
■ TACGTCCACTGGAGTCAC ■ TACGTCCACTGGACTCAC
■ RNA ■ RNA
■ AUGCAGGUGACCUCAGU   ■ AUGCAGGUGACCUGAGUG G
■ PROTEIN . PROTEIN
■ Met-Gln-Val-Thr-Ser-Val        . Met-Gln-Val-Thr-Stop _■ Examples: ß° thalasemia
	Gene mutations- types	
■	Normal state	■ Mutation type of trinucleotide
		expanse
■	DNA	■ DNA
	ATGCAGGTGACCTCAGTG	>    ATG(CAGCAGCAG] CAGGTGACCTCAGTG
■	TACGTCCACTGGAGTCAC	■   TAC(GT<          >TC] jo GTCC ACTGGAGTCAC
■	RNA	■ RNA
■	AUGCAGGUGACCUGAGUG	■    AUG(CA \G]2„CAGGUGACCUCAGUG
■	PROTEIN	■ PROTEIN
■	Met-Gln-Val-Thr-Ser-Val	■   Met ln]2„Gln-Val-Thr-Ser-Val
		■  Examples: Huntington's disease
Gene mutations- types
Gene mutations- types
■ Normal state a
■ DNA
■ ATGCAGGTGACCTCAGTG ■
■ TACGTCCACTGGAGTCAC "
■ RNA
■ AUGCAGGUGACCUCAGU
G ■
■ PROTEIN
■ Met-Gln-Val-Thr-Ser-Val
Mutation, type „frameshift"
DNA
ATGCAGGTGAACCTCAGTG TACGTCCAC TGGAGTCAC
RNA
AUGCAGGUGAACCUCAGUG
PROTEIN
Met-Gln-Val-Asn-Leu-Ser Examples:
Duchenn's muscular dystrophy, p° thalasemia,Tay-Sachs's disease
■ Normal state
■ DNA
■ ATGCAGGTGACCTCA GTG
■ TACGTCCACTGGAGTC AC
■ RNA
■ AUGCAGGUGACCUCA GUG
■ PROTEIN
■ Met-Gln-Val-Thr-Ser-Val
■ Mutation: type ..insertion"
■ DNA
■ ATGCAGGTG-30C
ACCTCAGTG
■ TACGTCCAC-30C
TGGAGTCAC
■ RNA
■ AUGCAGGUG-30C
ACCUCAGUG
■ PROTEIN
■ Met-Gln-Val----------------?
■ Examples: Hemophilia A
Gene mutations- types
Four basic types of heredity
Normal state DNA
ATGCAGGTGACCTCAGTG TACGTCCACTGGAGTCAC RNA
AUGCAGGUGACCUCAGUG PROTEIN
Met-Gln-Val-Thr-Ser-Val
Mutation: type ..deletion"
DNA
ATGCAGGTG TACGTCCAC
RNA
AUGCAGGUG
PROTEIN
Met-Gln-Val
Examples:
small-cystic fibrosis
large: Duchenn's muscular
dystrophy
Monogenic disorders
Monogenic disorders
■ Determined by one locus allele.
■ Variant allele which had arosen sometimes in the history replaces original („wild") allele on one (heterozygote) or both (homozygote) chromosomes.
■ Monogenic disorders have a characteristic transfer of the genotypes in families.
■ Rare alleles are associated with monogenic disorders as a „big" factor.
■ Clinical manifestations are observed usually in childhood.
■ Less than 10% are manifested after puberty and only 1% after reproductive age.
■ Prevalence about 0.36%; in 6-8% hospitalizod children some monogenic disorder is suspected.
Complex (multifactorial, multigene) diseases
■ They may be interactions of certain gene variants and certain environmental factors (and their combinations) which could be responsible for predisposition for many
■ biological processes
■ evol
■ O 2S.
> Genome and environmental factors can be changed by dii
> Genome is more im
Genome stability vs. genome variability
endangered during life time by many repeated DNA replications is preserved by different mechanisms.
y seems to be a source of surviving potenciál in changing environmental context.
Genome stability
■ Since our genomes are constantly exposed to e: id (e.g.
UV radiation) and
id (e.g. metabolically generated reactive oxygen species) D dar an impaired ability
to detect and/or respond appropriately to these efects can impact on the maintenance of genetic stability.
O'DrlscollM: CurrGenomics. 2008 May; 9(3): 137-146
Genome stability
■ There are many examples of human Mendelian disorders defective in the repair of or response to DNA damage.
■ The importance of these pathways is demonstrated by the increase in
in and
develoDmental abnormalities associated with these conditions.
O'DriscollM: CurrGenomics. 2008 May; 9(3): 137-146
Genome instability-copy number variants (CNVs)
Recent studies have revealed that DNA segments in sizes from kilobases to megabases can vary in copy number among individuals in a population.
These changes in copy number are the result of duplications, deletions, insertions, inversions and complex combinations of rearrangements, and are termed collectively copy number variants (CNVs).
van Attikum H, Gasser SM. Trends Cell Biol. 2009 May;19(5):20?-17.
Copy number variants
The changes in gene copy number are associated with different phenotypes in humans. Perhaps, the most well known example of this is the tn
Down syndrome.
An increased expression of the genes on chromosome 21 results directly or indirectly in a clinically heterogeneous disorder incorporating
impairment, facial dysmorphology, growth retardation, cancer predisposition, microcephaly, heart and skeletal abnormalities
Genomic disorders
Genomic disorders represent a clinically diverse group of conditions caused by g,
orientation of a genomic region containing
dosage-sensitive genes.
Determining how the o
(CNV) affects human variation and contributes
to the aetiology and progression of various
genomic disorders represents in
questions for the future.
O'Driscoll M: Curr Genomics. 2008 May; 9(3): 137-146
O'Driscoll M: Curr Genomics. 2008 May; 9(3): 137-146
Gene mutations as a cause of variability in genes
(prevalence  less  than   1% in population as a result of selection pressure and/or „recent" mutation). These mutations represent „great   genetic   factors" causing es-subjects of cli
s (prevalence more than 1% in population, smaller genetic factors in interactions with environmental factors conditioning - subjects of pe
Gene mutations as a cause of variability in genes
✓ are generating in somatic cells during the lifetime
✓ are cell and/or tissue specific, without transfer to offspring
■ Mutdtions in QGrm cells
•/ they    become    components    of genetic
predisposition s they are present in all cells of the individual
✓ they are transfered to offspring
Candidate gene and its association with disease
✓ The question is simplier in mendelistic diseases in which a change function of a gene can be easier indentified.
■ IWU 11 lall I possibilities for this strategy:
* Linkage analysis s needs examination of genealogy s is evaluating common occurrence of genetic marker and disease in related individuals
Genetic studies
■ Candidate
s Etiopatogenetic (pathophysiological) approach using for candidate gene selection
nalysis
s Based on analysis of large sequences of genome
Association studies
are evaluating common occurrence of genetic marker and disease in unrelated individuals
Types of association studies
□ case-control (healthy-ill)
? (severity of disease, early onset of disease, risk factors for disease including gender
□ genotype-phenotype   (e.g.biochemical parameters)
DNA markers
■ Thus, it is possible to associate alleles of many polymorphisms with clinical manifestation of the disease and/or with some phenotypes of a disease.
■ Therefore, a certain genotype and/or allele of the polymorphism can represent statistically higher flowed risk for the disease fodds ratioV
i
Odds ratio (OR):
Number of patients with risk genotype x number of healthy individuals with different genotype Number of healthy with risk genotype x number of patients with ottier than risk genotype
^ DNA marker does not have to be causative for the disease. Definitely, the most important characteristic of clinically useful DNA marker must be its high statistic asscociation with a disease and/or its phenotype.
Association of a disease with candidate gene variants: an example: I/D ACE
Fyhrquist F and Saijonmaa 0, Journal of Internal Medicine 264: 224-236, 2008
RPR, renin/prorenin receptor; Mas, mas oncogene, receptor for Ang 1-7; AT2R, angiotensin type 2 receptor
AT1R, angiotensin type 1 receptor, IRAP, insulin-regulated aminopeptidase; Ang IV receptor AMPA, aminopeptidase A;
AMPM, aminopeptidase M; ACE, angiotensin-con verting enzyme; ACE2, angiotensin-converting enzyme 2; NEP, neutral
endopeptidase.
Zygote      Embryo Adult organism
How does a single egg or zygote become a complete organism with many different tissues and differentiated cells?
How can this happen, when the zygote undergoes many rounds of mitosis — mitosis is supposed to produce identical daughter cells?
How do Organisms Control the Level of Gene Expression?
How do Eukaryotes Control the Level of Gene Expression?
■ Cells must only express genes when needed
■ Gene expression (transcription, translation) takes up large amounts of cellular energy and resources
■ Cells live frugal lifestyles — they conserve energy and resources
■ So genes will only be expressed when their products are needed.
■ Cells of more complex organisms turn on and turn off genes based on the functions of the cells — hence cells differentiate
■ Eukaryotes control genes at almost every level:
■ Regulation of Chromatin Structure
■ Regulation at the transcriptional level
■ Regulation at a post-transcnptional level
■ Regulation at a translational level
■ Regulation at a post-translational level
Regulation of Chromatin Structure
■ Histone acetylation prevents DNA from winding tightly around histones, allowing easy access to promoter sites (Deacetylation does the opposite)
■ DNA methylation causes DNA to wind tightly around histones, preventing easy access to gene promoters (Demethylation does the opposite)
Histones
Histone subunits are:
■ 2 units of H2A
■ 2 units of H2B
■ 2 units of H3
■ 2 units of H4
Histone HI is not in the core, but acts as a clamp and keeps the linker DNA in place Histones are positively charged, so DNA which is negatively charged, wraps around them
Bacteria lack histones, although some archea have them
Epigenetic Inheritance
Modification of chromatin does not change the DNA, only its expression.
However, this modification pattern IS inherited (remember genomic imprinting?)
Scientists now believe that certain environmental factors may play a part in promoting chromatin modification that causes expression or suppression of certain genes — e.g. one twin gets schizophrenia and another doesn't. Certain cancers may also be caused that way
Epigenetic effects
is
predominantly and has hi
levels of acetylated histone tails. Most mammalian transcription factors have GC-rich binding sites and many have CpGs in their DNA recognition elements.
Binding by several of these factors is impeded or abolished by methylation of CpG.
11
Regulation at the transcriptional level
■ Enhancers (proximal and distal)
■ Silencers
■ Transcription factors at promoters
■ General transcription factors
■ Specific transcription factors
■ All these play a role m regulating gene expression.
Enhancers increase the rate of a gene's expression and silencers decrease it
Transcription factors are needed if the gene is to be expressed at all.
Regulation at post-transcriptional level
RNA processing — alternative splicing allows certain proteins to be made instead of others (all from the same gene)
mRNA Degradation — cytoplasmic nucleases degrade mRNAs so polypeptide synthesis stops. More mRNA is made later, if necessary
5' caps and 3' tails can be removed or changed and this will prevent translation
Pre-translational Regulation
■ Certain proteins in the cytoplasm can bind to the mRNA's 5' UTR and prevent ribosomes from binding
■ Any change in mRNA shape will prevent ribosome binding
■ Decreased length of poly-A tail will prevent translation
Post-translational Regulation
■ Proteins can be ubiquitinzed and degraded in a proteasome
Non-protein-coding RNAs and Gene Regulation
■ MicroRNAs or miRNAs are small non-coding RNAs that were
■ Transcribed from DNA
■ Complexed with a number of proteins
■ These miRNAs have several bases that are complementary to some protein-coding mRNAs
■ The miRNA-protein complex can bind to these protein-coding mRNAs and prevent them from being translated
■ Nucleases eventually degrade the dsRNA
Cytoplasmic Determinants
■ Certain molecules such as maternal mRNAs, transcription factors and other proteins are localized in specific cytoplasmic regions of the unfertilized egg or zygote
■ These molecules affect cell fate decisions by segregating into different embryonic cells and controlling distinct gene activities in these cells (specialized transcription factors will only turn on certain genes).
■ Cytoplasmic determinants are also found in some post-embryonic cells, where they produce cytoplasmic asymmetry.
■ In dividing cells, this leads to asymmetric cell division in which each of the daughter cells differentiates into a different cell type. Also called localized cytoplasmic determinants or morphogenetic determinants.
Pharmaco-genetic
52
Cytoplasmic Determinants and Cell Fate
Pharmacogenetics & Pharmacogenomics
Pharmacogenetics & Pharmacogenomics
■ Pharmacogenetics: The role of genetics in drug responses.
o F. Vogel. 1959
■ Pharmacogenomics: The science that allows us to predict a response to drugs based on an individuals genetic makeup.
o Felix Frueh, Associate Director of Genomics, FDA
■ P cs: study of individual gene-drug interactions, usually one or two genes that have dominant effect on a drug response (SIMPLE relationship)
■ : study of genomic influence on drug response, often using high-throughput data (sequencing, SNP chip, expression, proteomics - COMPLEX interactions)
14
Relation to genes
■ Almost every pathway of drug metabolism, its transport or activation is influenced by genetic variability
■ Clinical variability in the response
■ The risk of side effects
■ Genotype specific dosage
■ Polymorphic targets drug
58
I - \ii\va
57
10 questions in polygenic disorders
s How important are genetic influences in the most common forms of
multigene diseases? ^ What is the influence of the environment on the onset of the disease? ^ Which are the most promising approaches to the determination of genetic
factors leading to the onset of disease? ^ Which genes have already been selected as candidate genes? ^ Which paths contribute to genetic susceptibility for the disease? ^ How many genes are involved in susceptibility to disease? ^ Are the most common forms of polygenic diseases associated with
frequent or rare genetic variability in the population? (hypothesis frequent
variations / frequent genetic disease vs. heterogeneous model) ^ Why alleles that are associated with the disease were not eliminated from
the population?
^ The importance for the disease-environment interaction genes and genes-genes?
What are the implications for pharmacogenetics?
60
Genetic polymorphisms in drug	
metabolizing enzymes	
Fhntl	-CVP1A1I2                            Phase II r^'6' NATS
	CYP2B5                                                  ^ GST-M /        - f>'r.
a,i,„- J	
	LtGTe V\
	CYP?E1 *"cOUT rpivrr
From: Evans WE, Relling MV. Pharmacogenomics: Translating functional genomics into rational therapeutics. Science 286:487-491, 1999. 59
15
Pharmacogenetics: A Case Study
Pharmacogenetics: A Case Study
Pharmacogenetics: A Case Study
Clinically relevant genetic polymorphisms in relation to the side effects of drugs
Clinically relevant genetic polymorphisms in relation to the effectiveness of drugs
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Glucose-6-phosphate dehydrogenase activity
Drugs and Chemicals Unequivocally Demonstrated to Precipitate Hemolytic Anemia in Subjects with G6PD Deficiency
Acetanilide        Nitrofurantoin Primaquine
Methylene Blue   Sulfacetamide Nalidixic Acid
Naphthalene Sulfanilamide Sulfapyridine Sulfamethoxazole
67
Effects >100 million worldwide
-C^E-► R-NOH
R-
NH,
MPO PGH Synthase
ERYTHROCYTE
NADP+ or
\f GSSG(?)^ R-NOH ^ H9bFe
NADH
2 NAD+
Sr
tA NADPH A R.N0  <A> HgbFe^A*6' orGSH(?)^ J
GSH      Reactive _^ Splenic
Semi-mercaptal Oxygen Sequestration
1
sulfanamide
R-
NH2
Detoxification
Hemolytic Anemia
INCIDENCE OFG6PD DEFICIENCY IN DIFFERENT ETHNIC POPULATIONS
Ethnic Group Incidence(%) Asiatics
Chinese	2
Filipinos	13
Indians-Parsees	16
Javanese	13
Micronesians	<1
Iranians	8
Greeks	0.7-3
Persia	15
Cytochrome Oxidase P450 Enzymes
■ 57 Different active genes
■ 17 Different families
■ CYP1, CYP2 and CYP3 are primarily involved in drug metabolism.
■ CYP2A6, CYP2B6, CYP2C9 .CYP2C19, CYP2D6, CYP2E1 and CYP3A4 are responsible for metabolizing most clinically important drugs
Polymorphic	CYP2B6			CYP2C9		
Cytochrome P-450s	-ul-lr......		:z::z........-			
	iHIPttHAXI ■>=.;-■-. >|jl I-Halts mid*	OnnMM is	3(:i of CnrJMM	WS I HypogiywHiif ARBl IrbMdrtan ItaanM		14« i.....>l ■ ■•
						
		CYP2C1&			CYP2D6	
						
	selected             .    bl               ma Meta&oiüer L«J,"H' leiden«					
	Frettjn pump H AmrtriptyHne QNl• ■[ifi-■■■::"i imidi diuefum phe-rtdurbilal	CJiromonMrifr 10	15-30^ Allan*	■       -: ■- - : -(hlwohtnlraniln* rf<iHtrrnnrtrtfiiprinn «idsnulrofi lidneiint iBomfitaiinp	OthHMMM iJ	
				© 2006 Americ	n Medical Association. All rights r	
Effect of Metabolic Rate on Drug Dosage
Poor Metabollzer Ph&notype
Prodrug, needs metabolism to work (eg, codeine K metabolized by CYP2D6to morphine) Active drug, inactivated by metabolism (example i-s omeprazole)	Poor efficacy Possible accumulation of prodrug Good efficacy Accumulation of active drug can produce .adverse reaction; May need lower dose
	
D,u,	Ultra-rapid Metabollzer Phenotype
Prodrug, needs metabolism to work (eg. codeine a metabolized by CYPZHto morphine)
Active drug, Inactivated by metabolism (example is omeprazole)
Good efficacy, rapid effect
Poor efficacy
Need greater dose or slo\
release formulation
Debrisoquine phenotype in subjects with different CYP2D6 genotypes
Genotvoe	#of	Metabolic
	Subjects	Ratio
CYP2D6wt/(CYP2D6L)2	9	0.33
CYP2D6wt/CYP2D6wt	12	1.50
CYP2D6wt/CYP2D6(A or B)	9	2.14
CYP2D6B/CYP2D6B	6	48.84
Data from: Agundez JG et al. Clin Pharmacol Ther 57:265, 199,5.
Codeine and Cytochrome P450 CYP2D6
■ Codeine is a commonly used opioid
■ Codeine is a prodrug
■ It must be metabolized into morphine for activity
■ Cytochrome P450 allele CYP2D6 is the metabolizing enzyme in the liver
■ 7% of Caucasians are missing one copy of the Cytochrome P450 CYP2D6 gene
■ codeine does not work effectively in
thp^p individuals
Why Maintaining Warfarin Therapeutic Range is Critical
European Atrial Fibrillation Trial Study Group, N Engl J Med 1995;333:5-10.
Estimated Warfarin Dose (mg/day) Based on Genotypes
CVPZC9 genotype
		*l/*2	*l/*3	*2/*2	*2/»3	*3/*3
66	6	5	4	4	3.5	3
GA	©	4	3	3	2.5	2
AA	3	2.5	2	2	2	1.5
'Kim MJ, Huang S-M, Mcytr U, Batman, A. Lesko LT.
CYP2C9 ACTIVITA
5.63 (2.56) *1/*1
4.88 (2.57) *l/*2
3.32 (0.94) *l/*3
4.07 (1.48) *2/*2
2.34 (0.35) *2/*3
1.60 (0.81) *3/*3
From: Higashi MK, et al. Association between CYP2C9 genetic variants and anticoagulation-related outcomes during warfarin therapy. JAMA 287:1690-1698, 2002. 78
Frequency of VKORC1 Alleles
in Various Populations
-1639 &>A AA	AG	6G
Caucasians 19% (N=297)	56%	25%
Spanish 32% (N=105)	40%	28%
Chinese ^80£) CN=104)>Wj--	18%	2%
African ^^^% Americans fcfch-(N=159) ■E^KE	21%	79%
Another Anticoagulant Clopidogrel (Plavix) and CYP2C19 Alleles			
	u	)*.r>rtiŕ Rnporic Cop.dogFíl. )D0 mi	
	I,o	T	
	] 5	■ 1 ! . -	
		■ i 1 UM       EU       lU N N-M)   IN-11)   (N-W) (N>1)	
PM: with two reduced function alleles IM: one reduced function allele EM= no variant alleles; UM. one or two "17			
Interaction with drogs metabolized and/or reactingi with CYP2C9
Competition	Enzyme inductor	Enzyme inhibitor
ASA a většina_	rifampicin	fluvoxamin (ostatní SSRI slabí)
fenobarbital, fenytoin	fenobarbital, fenytoin	
S-warfarin	karta mazapin	inhihitniy UMft.P.ftA rarinletáry
losartan		tolbutamid
tolbutamid		Cimetidin (slabý)
sulfonamidy, dapson		aTfilnva amimyfcfitika (slabá)
diazepam, tenazepam		ritonavir
fluoxetin, moclobemid		desethylamiodaron
zidovudin		
GENETIC POLYMORPHISMS, MATERNAL SMOKING AND LOW BIRTH WEIGHT (LBW)
65% of all infant deaths occur among LBW infants, while LBW infants account for 7.6% of all live births
Reduction in birth wgt among smoking women
Genotype CYP1A1 AA CYP1A1 Aa/aa
Weight Reduction 252 g 520 g
GST1 AA/Aa 285 g
GST1 aa_642 g
Data from: Wang X, et al. JAMA 287:195-2002, 2002.
Metabolic rate
b) Geneticky polymorflzmus
According to the activity of the enzyme may be a population divided into four main groups - poor metabolisers (PM), intermediate metabolizers (IM), efficient metabolizers (EM), and ultra-fast metabolizers (UM).
Mostindividuals among the white population - extensive metabolizers (EM) - the drugs are metabolized by the expected rate.
5-10% of individuals are genetically determined poor metabolisers (PM) - the slow degradation of substances metabolised and are at a higher incidence of adverse events.
Intermediate metabolizers (IM) are represented in 10-15% and in long term treatment in response — comparable to PM.
Ultra-fast metabolizers (UM) — metabolization is intensive; clinically unresponsive to the usual doses of drugs - 5-10%.
Ultrarychli metabolizátori Rychlí metabolizátori Intermediární metabolizátori Pomalí metabolizátori
Meta holická aktivita eiizvmu
21
Methotrexate in RA
■ Effectiveness of treatment of rheumatoid arthritis (RA) by methotrexate (MTX) 46% - 65% (ACR20)
■ During treatment with MTX side effects may occur. At least one in 72.9% of patients, severe in 30% of patients.
gastrointestinal toxicity (nausea, vomiting, diarrhea, 20% - 65% Hepatotoxicity 10% - 43% oral ulceration 37% alopecia to 4%
■ pulmonary toxicity 2.1% - 8%
■ Bone marrow suppression light 12%
■ pancytopenia 0-8%
86
Methotrexate
Methotrexate
T
Folate
Methotrexate
Folate
Active-Iransport process
Dihydtofolate ...... Methotrexate
reductase
dTMP
dUMP
Ns, N,0-Methylene-FH4
Folic acid not useful in toxicity
Folinicacid N5 formyl FH, should be given which is converted to N5,N10-Methylene -FH, and bypasses the inhibited reductase
Adenine, guanine, thymidine, methionine, serine
( lini.jl cllci.1i
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Ranganathan P, McLeod HL. A&R 20
Methotrexate
Halt ■ MTX p»lny I1- K n - i^n,- -n I r:.-. .-. an pen frudlKtn
I ] II, Ji . II, 11 ■
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MS         MufnUt.in ..| hnvyMnw     M1%G May draow US ■intf)
MIRK      McHnblmn nl .<M« AMC ^.      ■! rtqtMrrd fiv the
ms
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Mil dnw MIRK KlnHf.        May died MTX hnxMi HI. fC
Ranganathan P, McLeod HL. A&R 20*
MDR1
MDRl (ATP-binding cassette Bl/multidrug resistance 1) is
an efflux pump that transports toxic endogenous
substances, drugs and xenobiotics out of cells.
It is known to affect susceptibility to many hematopoietic
malignancies.
ABCB1/MDR1 polymorphisms may either change the protein expression or alter its function, suggesting a possible association between ABCB1/MDR1 single nucleotide polymorphisms (SNP) and clinical aspects of T-cell lymphoma.
Therefore, association of two polymorphisms in the gene with clinical staging and therapy was evaluated.
(A) An example of an experimentally verified miRNA pharmacogenomic set. miR-125 b inhibits vitamin D receptor (VDR) expression.
Why are some gliomas resistant to nitrosourea
Evidence suggests this may be the result of an epigenetic phenomenon - one that does not involve a change in DNA
^EmB^I^I    MGMT - methylguanine-DNA
region of MGMT may silence the gene
From: Esteller M, et al. Inactivation of the DNA-repair gene MGMT and the clinical response of gliomas to alkylating agents. NEJM 243:1350-1354, 2000. 93
	
Glioma with unmethylated MGMT MGMf promote!   1   Exonl Inlionl	OS. Co Alkyl group removed by MGMT from the ON A base guanine
Glioma with methylated MGMT Methyl MGMTpiornotel Gsne inagbvailon	Carmustine cross-links DNA strands, and There is no aclive MGMT to repair it
24
FDA Requires Genetic Tests for Certain Therapies
List of FDA Required or Recommended Biomarker Tests in Drug Labels
Eiuntirkcr	Tciil>	Drug Eximpk	1 >l-i Pil^ilIltll-l (n-».l million)
CTP2C9	ReconiLUciKted	Warfarin	
		(_ LLllAilll.il)	
G6PD deficiency	Eecommttid-eil	Diipsnm	D 0231
l..I-J 'L"> lUlllltll^	ül-c^mtTAttMltil	K.t-''iui-..i-<	0.0000
			
overex]>K5sloii		Trwrnnimih	0.0003
TPMT VLiriiLciii	JiL-mTimtriUi'il	.\.,nk:i'|Tiiv.	0.1 IAS
rPMIvarLitits	RcL^mtut tided	M I-     i ■ ■ ■ i. -	L'.-HI
TPMT Variants	llLLi>]iirTicndc-d	[ luo^Li.uuiii:	0.0C12
IICTIAI ■—-	Rr-nnrn mended	IruiiiM'r.iii	0.0002
Urea cycle			
enzyme deficiency	k.cc4.hh mended	\alprak acid	■ \h
T- -i. .■ 1			2.766
CVP = iyiLnhiuiii* f4W, t.tit-K = human ijiUtiniLiL |jii-»[h Ittvti rttepi pJiosphale drhydiogLiu». HEfli/iitu ■ human rpldctuiaL growth held			r. G4PD = gkKUt-4-K-LtLMOI   J    1 I'M .
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