ASCP Technologist in Molecular Biology board exam prep
Optimization of PCR methods
1. Check the Tm 2. Mg2+ concentration - too little can result in no PCR product, and too much may produce noise 3. PCR cycles 4. Add, extend, or increase the temp of the initial template denaturation step 5. Concentrations of other buffer components 6. GC Content
Pre-transplant evaluation
1. Determine HLA type: Serology 2. Determine serum Ab status: CDC, sequencing 3. Crossmatch: MLC, CDC, ELISA, flow cytometery
NASBA steps
1. Hybridize oligo-T7P primer to target seq 2. RT/RNase H 3. Hybridize with target-specific oligo primer (P2) 4. RNA transcript of T7 RNA pol
Thermal Cycling steps in conventional PCR
1. Initialization (94-96 C) 2. Denaturation (94-98 C) 3. Annealing (50-65 C) 4. Extension (70-80 C) 5. Repeat 2-4 ~30x 6. Final Elongation (70-74 C) 6. Final hold
What are the steps in DNA replication?
1. Initiate 2. Elongate 3. Terminate
Line Probe Assay steps
1. Isolate nucleic acid (RNA) 2. Amplify 3. Hybridization 4. Strigent wash 5. Incubate with conjugate 6. Incubate with substrate 7. Detect
Solid phase isolation
1. Lyse 2. Acidify (low pH) 3. Transfer to column (adsorption) 4. Wash 5. Elute
Inorganic isolation
1. Lyse 2. Add low pH/high salt soln (NaOAc ppt's proteins) > vortex/spin 3. Transfer soln to new tube 4. EtOH ppt 5. Resuspend
Organic isolation method
1. Lyse 2. Add phenol/ chloroform > vortex/spin 3. Transfer aqueous layer (top) to new tube 4. Add chloroform:IAA (removes phenol) > vortex/spin 5. Transfer aqueous layer to new tube 6. Add NaOAc and EtOH > vortex/spin 7. Decant 8. Resuspend
Heterduplex Analysis steps
1. PCR 2. Mix sample and CTR DNA together 3. Denature PCR using heat 4. Cool slowly to rt 5. Add denaturing loading buffer 6. Run on MDE gel
PCR process
1. Prep MMx: buffer, taq, primers, dNTPs 2. Add target 3. Place in thermocycler 4. Denature dsDNA 5. Anneal: allows primers to hyb 6. Extend: pol adds dNTPs to 3' 7. Repeat steps 4-6
Bisulfite DNA sequencing/Methylation specific
1. RE digest 2. Electrophorese and purify fragment of interest 3. Denature and incubate w/ sodium bisulfate (turns C>U, methylated C is unchanged) 4. clean, ppt, and resuspend 5. PCR --> sequence 6. Compare treated vs untreated, note where CG are not changed to TA
Southern Blotting Procedure
1. RE digest DNA 2. Gel electrophoresis 3. Soak in HCl (depurinates, weakens H-bonds) 4. Soak in NaOH (denatures) 5. DNA transferred to a membrane 6. Immobilize (UV or bake) 7. Pre hyb to block 8. Hyb with probe
Southern Blot steps
1. RE digest to fragment DNA 2. Run on gel to separate 3. Soak gel in alkali/NaOH to denature dsDNA 4. Transfer ssDNA fragments to positively charged membrane (blot) 5. Fix to filter by heat (80C) or UV crosslink 6. Incubate (hybridize) blot w/ radioactively labeled ssDNA comp probe 7. Autoradiograph
Pulse Field Gel Electrophoresis steps
1. culture 2. embed pellet in agarose plug 3. treat w/ lysozyme (cell lysis) 4. proteinase K 5. gel
Microarray steps
1. isolate mRNA from cells 2. RT to get labeled cDNA copies of mRNA 3. cDNA washed over slide. cDNA sticks to comp sequence 4. use laser to read fluorescent tags
Describe the steps of reverse transctiption
1. tRNA acts as a primer and hybridizes to virus genome 2. Complementary DNA then binds to the U5 (non-coding region) and R region 3. RNAse H degrades the 5' end of the RNA which removes the U5 and R region. 4. The primer then "jumps" to the 3' end of the viral genome and the newly synthesized DNA strands hybrid
Calculate the RNA concentration from the following: 260=0.307 (DF 1:100)
1228 ug/mL = 0.307 abs * 40 ug/mL * 100 DF
Von Willebrand dz (vWD)
12p13, Von Willebrand's factor (vWF) vWF promotes platelet clumping Mutations effect bloods ability to clot
Breast cancer, Brca2
13q 6174delT TS; interacts w/ RAD51
Nucleosome
147 bp of DNA wrapped around histone octamer plus a H1 linker
Tay Sachs disease
15q, HEXA gene; AR 1278insTATC, exon 11 Insufficient hexoaminidase A activity; GM2-gangliosides cannot be broken down and accumulate in the brain; causes cerbral degeneration and blindness
Breast cancer, Brca1
17q 185delAG/187delAG 5382insC/5385insC TS; interacts w/ RAD51 (DNA damage repair)
Breast cancer, Her2/Neu/ErbB2
17q, ErbB2; proto-oncogene, Tyr kinase Mutations cause overexpression -> proliferation Dx: IHC, FISH, qPCR Treatment: Transtuzumab (Herceptin), gefitinib (Iressa)
Methylenetetrahydrofolate reductase
1p36.3, MTHFR gene; C677T (A222V), A1298C (E429A) Methylenetetrahydrofolate reductase catalyzes conversion of MTHF--> 5-MTHF which is converted to Met Thromboembolism, homocysteine builds up, Met is depleted
Gaucher's disease
1q21 GBA; AR N370S or L444P Lipid, glucosylceramide, accumulates in WBCs, liver, spleen, lungs, bone marrow and, less commonly, brain, caused by a deficiency of the enzyme glucocerebrosidase, which helps the body process the fatty substance glucocerebroside. Dx: PCR ->seq coding region
Factor V Leiden
1q25, F5 gene 1691G>A, R506Q Causes deep vein thrombosis Treated with anticoagulants (warfarin/Coumadin)
Strand Displacement Amplification (SDA)
1st stage: target generated w/ RE site 2nd stage: probe amp; HincII nicks at RE site, DNApol extends/regenerates RE site and displaces strand high throughput high sensitivity
Hybridization
2 ssDNA molecules of comp base sequence can form a ds hybrid (duplex)
Human genome
2.9 billion bp ~30k - 40k genes 46 chr, diploid
How do you inactivate RNases?
200C for 2 hrs 30 min in 1M NaOH or quanidinum isothiocyanate
At what wavelength does DNA and RNA absorb?
260 nm
At what wavelength does protein absorb?
280 nm
What is the wavelength for background in spectrophotometery?
320 nm
[DNA] = 767.5 ug/mL. You have 0.5 mL What is the total yield.
383.75 ug = 767.5 ug/mL * 0.5 mL
Quaternary protein structure
3D structure of a multi sub unit protein
Tertiary protein structure
3D structure of a single protein
Bart's hydrops fetalis
4 α genes deleted, --/-- γ4 present, fatal in utero
[DNA] = 860 ug/mL. You have 0.5 mL. What is the total yield.
430 ug = 860 ug/mL * 0.5mL
How do you determine quality of DNA/RNA using a spectrophotometer?
A260/A280
Start codon
AUG (Met)
What is the path of a tRNA in a ribosome?
Acceptor > Peptidyl > Exit
DNA Polymerase β (Euk)
Base excision repair (BER)
Single-strand conformation polymorphism (SSCP)
Based on the preference of DNA to exist as DS rather than SS; Forms 3D conformers - a SNP can cause the conformer to fold differently (kinks, loops, bubbles, and tails)
Telomeric probes
Best for cryptic translocations or small abnormalities
Break apart probes
Bind to the chr flanking the t breakpoint region WT will emit a combination signal (next to each other) and t will emit separated signals.
single-strand DNA binding proteins (SSBPs)
Binds ssDNA and prevents it from re-annealing during TXN, replication, repair, and recombination
Hazard label
Blue: Health hazard Red: Fire hazard Yellow: Reactivity White: specific hazard 0 no hazard - 4 severe hazard
Helicase
Breaks H-bonds of double helix at the replication fork
DNA Polymerase IV (Prok)
Bypass replication SOS response
DNA Polymerase V (Prok)
Bypass replication SOS response Translesion synthesis DNA repair
PCR DNA Array
DNA array is a collection of spots attached to a solid support (such as a microscope slide) where each spot contains one or more ssDNA oligo fragments. Arrays make it possible to put down large quantities of very small spots on a single slide. Each spot has a DNA fragment that is complementary to a single DNA sequence.
RNA polymerase
DNA dependent RNApol Transcribes DNA template to RNA (3'-->5'; anti-parallel)
Southern Blotting
DNA is isolated and cut with REs. This allows investigators to determine the molecular weight of a restriction fragment and to measure relative amount in different samples.
After an extraction/isolation, what should you elute with?
DNA - TE or water RNA - DEPC water
FRET probes
Fluorescence Resonance energy transfer - Distance dependent interaction between the electronic excited states of two dye molecules in which excitation is transferred from a donor molecule to an acceptor molecule without emission of a photon.
Calculate the Tm of the following primers: Forward: GGAGCTTTGTTTCAACCAAG Reverse: ATTAAATGCGGAATTGCCCA
Forward: Tm=(4C x 9GC)+(2C x 11AT) = 58C Reverse Tm=(4C x 8GC)+(2C x 12AT) = 56C
Dye primer
Four different fluorescent dyes are added to the primers. Cycling is done to attach the primer and that is what the instrument sees. Each nucleotide is amplified a different color.
DNA Polymerase III (Prok)
Primary enzyme involved in replication Exonuclease activity
DNA Polymerase α (Euk)
Primase DNA dependent DNA & RNA pol
What are some causes of too many bands on a gel after PCR?
Primers not specific Annealing temp too low Too many cycles Too much Mg++
A small portion of chr 2 has been found on the end of chr 15 and a small portion of chr 15 was found on the end of chr 2. This mutation is called a:
Reciprocal translocation
How can Tween 20 affect PCR?
Stabilizes Taq Suppress formation of 2* structures Increase yield Increase non-specific amplification
Why is the lectin, phytohemagglutinin (PHA), added to a cell culture when preparing cells for karyotyping?
Stimulates mitosis in the cells
For long term storage, what should you store DNA in?
TE or DNase free H2O
Microarrays
Used for unknown gene and mutation cDNA libraries can be used for gene expression, tumors, genetic mapping, mutations and polymorphism large scale, high throughput analysis
Sequence Based Nucleic Acid Amplification (NASBA)
Used to amplify RNA sequences; Primer-dependent technology that can be used for the continuous amplification of nucleic acids in a single mixture at one temperature; works at 41 C
Reverse Transcriptase PCR
Used to detect RNA expression levels. RT-PCR is used to qualitatively detect gene expression through creation cDNA transcripts from RNA.
In-situ hybridization
Used to detect protein, RNA, and DNA within the cell. Probes bind to the DNA and can be visualized under the microscope. Depending on the mutation, different signals can be seen - deletions and duplications. Sensitivity can be increased by using dual fusion probes, break apart probes, centromeric probes, and telomeric probes.
Restriction fragment length polymorphism (RFLP)
Used to detect sequence alteration in retriction enzyme fragments; The region surrounding the mutation is amplified and the mutation is detected by cutting the amplicon with the correct restriction enzyme
Interphase FISH
Used to study prenatal samples, tumors, and hematological malignancies Cells do not have to be cultured Fix cells Hyb to probe (dual fusion, break-apart, CEN, telomere)
Metaphase FISH
Used to study smaller abnormalities Culture cells for 72 hrs Add colcemid to arrest cells in metaphase Fix Hyb to probe (chr paint)
Fluorescent in situ hybridization (FISH)
Uses fluorescent probes to detect DNA sequences on chr
IonTorrent sequencing (NextGen)
Uses standard sequencing chemistry, but a semiconductor based detection system. Based on the detection of hydrogen ions that are released during the polymerization of DNA as opposed to the optical methods. A microwell containing a template DNA is flooded with a single type of nucleotide (A,T,G,C) and if the nucleotide is complementary to the template it is incorporated into the growing strand of DNA. This causes the release of hydrogen ions that triggers the sensor.
Dual fusion probes
Uses two pairs of probes with different fluor dye Bind regions that span the breakpoint of both t partners If t is present, signal from both dyes should be present
lab developed tests (LDT)
a term used to refer to a certain class of in vitro diagnostics (IVDs). In the United States, the Food and Drug Administration has determined that while such tests qualify as medical devices, FDA will allow these products to enter the market without prior approval from the Agency.
Blocking Proteins (Hybridization)
minimize nonspecific binding of probe to membrane ie casein (milk), Denhardt's sol
Blocking DNA (Hybridization)
minimizes probe binding to nonspecific sequence ie salmon sperm DNA, Human LINE-1
Splicing
modification of the nascent pre-messenger RNA (pre-mRNA) transcript in which introns are removed and exons are joined.
DNA Polymerase γ (Euk)
mtDNA replication and repair Exonuclease activity
Haemophilia
X, XR Blood does not clot due to a deficiency in a coag factor Haemophilia A: most common, factor VIII deficiency
Muscular dystrophy (DMD/BMD)
Xp21, dystrophin gene; XR Causes muscle weakness and muscle loss DMD: non-functional protein made BMD: some function of protein is retained
Fragile X syndrome
Xq27 FMR1, CGG repeat 5' UTR causes methylation Mental retardation WT repeats 5-55, carrier 56-200, mutation 200-2000+ Dx: PCR, S. blot for full mutation
Should you lyse RBCs before freezing?
YES
What some causes of DNA damage?
mutagens carcinogens cell death age-related decreases in DNA repair genetic disease
What would the autoradiogram show if the stringency was to high?
no bands
Eupliod
normal complement of chromosomes
ORI sites
nt sequence where replication is initiated
Clinical sensitivity and specificity is based on _________.
outcome
What is the function of rRNA?
part of ribosome structure most abundant RNA coordinated coupling of tRNA to mRNA codons
An RNA preparation has the following readings: 260=0.208 280=0.096 Is this RNA suitable for use?
Yes, 2.17 is suitable for RNA analysis A260/A280 = 0.208/0.096
Do you have to know the gene sequence in order to do DNA sequencing?
Yes, in order to design primers You do NOT need to know the mutation
Polymorphism
a change in the DNA sequence that is present in at least 1-2% of the population (ex. Sickle cell anemia)
Solenoid
a coil of six nucleosomes wound into a tightly packed helix
Pleiotrophy
a single gene controls the expression of many phenotypic traits ie Sickle Cell Anemia
Huntington disease (HD)
4p16.3 HD/HTT; CAG repeat CAG repeat in HD/HTT causes multiple Q's at 5' of Huntingtin protein. Protein aggregates in plaques (especially in nervous tissue) slowing down brain function; symptoms appear at 30+ yo; impaired judgement, slurred speech, difficulty swallowing, intoxicated appearance WT repeats 9-37, HD 38-86 repeats Dx: PCR, S.blot to resolve full mut
5' cap
5'-5' pyrophosphate bridge to a methylated G added to 5' end of a mRNA Protects against degradation and as a recognition signal for TLN apparatus
Hereditary hemochromatosis
6p21.3 HFE; C282Y, G>A; AR a genetic disease that causes the body to absorb and store too much iron Treatment: phlebotomy
[DNA] = 1535 ug/mL. You have 0.5 mL. What is the total yield.
767.5 ug = 1535 ug/mL * 0.5mL
Cystic fibrosis (CF)
7q31.2 CFTR gene; F508del; AR Cl channel membrane protein Affects cells that produce mucus, sweat, saliva, and digestive juices; causes thick secretions Dx: RFLP, PCR-RFLP, HD, Invader, SSP-PCR
Calculate the DNA concentration from the following: 260=0.172 (D.F. 1:100)
860 ug/mL = .172 abs * 50 ug/mL * 100 DF
What is considered poor quality RNA/DNA from spectrophotometry?
<1.7 Protein contamination
Acrocentric
A chr where the with a centromere not in the middle, but closer to one end or the other
Hemoglobinopathies
A group of inherited disorders in which there is abnormal production or structure of the Hb molecule. Such disorders include hemoglobin C disease, hemoglobin S-C disease, sickle cell anemia, and various types of thalassemia.
Histocompatibility
A state or condition in which the absence of immunological interference permits the grafting of tissue or the transfusion of blood without rejection.
Bisulfate DNA sequencing
A type of chain termination sequencing designed to detect methylated nucleotides. Methylation of cytosine residues in DNA is an important part of gene regulation and expression - this is important for detecting different types of cancer. During the incubation C is converted to U and 5-methylated C is unchanged. A PCR reaction is then performed using normal chain termination methods.
research use only (RUO)
According to FDA, manufacturer-initiated studies of RUO products are typically intended to evaluate design, limited-scale performance, and issues such as usability of the test. The agency acknowledges that RUO products may be used for non-clinical laboratory research for goals other than developing a commercial IVD product. According to FDA, these uses may include developing novel and fundamental medical knowledge related to human disease and conditions.
Chromosome mutations
Affects the structures of the entire chr, requires the movement of large chr regions
What does the incubation step in hybridization do?
Allows formation of ds molecules
Secondary protein structure
Amino acids are linked by H bonds to form sub structures; eg a helixes, B sheets
The Joint Commission
An independent, not-for-profit organization, The Joint Commission accredits and certifies more than 20,000 health care organizations and programs in the United States. Joint Commission accreditation and certification is recognized nationwide as a symbol of quality that reflects an organization's commitment to meeting certain performance standards.
Sickle cell anemia
An inherited blood disorder where RBCs form a rigid disc or crescent shape HbS: β6Glu>Val HbSS: sickle cell anemia
Thalassemias
An inherited blood disorder where the body makes an abnormal form of Hb, the protein in RBCs that carries O. The disorder results in excessive destruction of RBCs --> anemia. Mutations or del of the α or β genes
Denaturing High-performance Liquid Chromatography (HPLC)
Analysis for PCR products 150-450 bp. The heteroduplexes elute ahead of the homoduplexes as the conditions intensify. The migrating homoduplexes are detected by absorbance at 260nm or fluorescence.
Warfarin (Coumadin)
Anticoagulant, prevents thrombosis thromboembolism VCORC1: -Group 1: fast metabolizers/high dose -Group 2: slow metabolizers/low dose CYP2C9: SNPs cause slow metabolism/low dose
Clopidogrel (Plavix)
Antiplatelet agent Activated by CYP2C19 CYP2C19 poor metabolizers at high risk of treatment failure, death, heart attack, and stroke
Post transplant lymphoproliferative disorder (PTLD)
B-cell proliferation due to therapeutic immunosuppression after organ transplantation following infection with Epstein Barr Virus. Patients may develop infectious mononucleosis-like lesions or polyclonal polymorphic B-cell hyperplasia.
Crossmatching
CDC is used to crossmatch potential donor and recipient Recipient serum is the source of Ab tested against donor lymphocytes
What is the function of tRNA?
Carries aa to ribosome Anticodon pairs with codon on mRNA strand
What is the function of mRNA?
Carries genetic info out of nucleus Transcript translated to protein
DNA polymerase
Catalyzes phosphodiester bond between nt's Uses ssDNA as a template to determine which nt's to add
BK virus nephritis (BKVN)
Caused by BK virus (BKV) in renal transplant recipients Use of immunosupressent drugs allows BKV to replicate w/i graft, causing BKVN resulting in graft failure for many
Genome mutations
Change in the number of chr's
Multilocus sequence typing (MLST)
Characterizes bacterial isolates by using sequences of internal fragments of housekeeping genes (6-7, 450-500 bp)
Which pathogens can LCR be used to detect?
Chlamydia Gonorrhea Listeria HPV Sickle cell dz
Endonucleases (Euk)
Cleaves phoshpodiester bonds w/i poly-nt chain DNase I: induces DSBs AP endonuclease: BER
CLSI
Clinical Laboratory and Standards Institute; A not-for-profit membership organization, the Clinical and Laboratory Standards Institute (CLSI) brings together the global laboratory community for a common cause: fostering excellence in laboratory medicine. We do so by facilitating a unique process of developing clinical laboratory testing standards based on input from and consensus among industry, government, and health care professionals.
Ligase
Closes gaps in DNA Catalyzes phosphodiester bond between 3'OH and 5'P
Nucleic Acid labeling
Common labels used to generate nucleic acid probes include radioactive phosphates, biotin, fluorophores and enzymes. In addition, the bioconjugation methods used for nucleic acid probe generation may be adapted for attaching nucleic acids to other molecules or surfaces to facilitate targeted delivery or immobilization, respectively.
HLA class III
Complement C2, C4, B Expressed on plasma proteins
Splicesomes
Complex of snRNPs Removes introns from pre-mRNA and splices exons together
How are nucleotides joined together?
Condensation to form phosphodiester bond
CLIA
Congress passed the Clinical Laboratory Improvement Amendments (CLIA) in 1988 establishing quality standards for all laboratory testing to ensure the accuracy, reliability and timeliness of patient test results regardless of where the test was performed.
Illumina sequencing (NextGen)
DNA molecules and primers are attached on a slide and amplified with polymerase to form DNA clusters. Four types of reversible terminator bases (RT-bases) are added an the non-incorporated nucleotides are washed away. Images are taken of the fluorescently labeled nucleotides as the sequence extends, then the dye, along with the terminal 3' blocker allowing for the next cycle to begin.
DNA Polymerase II (Prok)
DNA repair, exonuclease activity
Mutation
DNA sequence change that is present in a relatively small proportion of the population <1%, somatic changes
Components of PCR
DNA template Two primers that are complementary to the 3' Taq polymerase dNTPs Buffer solution Mg2+ (divalent cations) - higher Mn2+ concentration can increase the error rate during DNA synthesis
What is considered good quality DNA/RNA from spectrophotometry?
DNA: 1.7-2.0 RNA: 2.0-2.3
Terminal transferase
DNApol synthesizes poly-nt chain at 3' end w/o a template
Primase
DNApol α (DNA dep RNA pol) adds short segments of complementary RNA to ssDNA template (primers), serves as starting points for replication
Exonucleases
Degrades nucleic acids by removing one terminal nt at a time Cleaves phosphodiester bond at end of chain 5' --> 3' and 3' --> 5'
Exonuclease I
Degrades ssDNA from 3'-->5'
Exonuclease VII
Degrades ssDNA from either the 5' or 3' ends One of the few enzymes with 5' exonuclease activity.
What is the genetic abnormality of: 46, XX, del(22q11.2)
Deletion in region 1, band 1, sub-band 2 of the long arm of chr 22 (diGeorge's syndrome)
What is the genetic abnormality of: 46,XY,del(16p14)
Deletion in region 1, band 4 of the short arm of chr 16
What can Southern Blots be used to detect?
Deletions/insertions Point mutations Polymorphisms Structural rearrangements
What are the 3 steps of PCR and their temperatures?
Denature 90-96C Anneal 50-70C Extension 68-75C
Southern Blot
Detect a large DNA fragment among many Target: DNA, probe: DNA
What can inhibit PCR amplification?
Detergent (SDS) Phenol (left over from DNA isolation) Heparin (specimen tube) Heme Dyes CSF, urine, sputum, parafilm
Mixed leukocyte culture (MLC)
Determines T-cell cross-reactivity donor and recipient lymphocytes are mixed in culture; the degree of incompatibility is indicated by the number of cells that have undergone transformation and mitosis, or by the uptake of radioactive isotope-labeled thymidine.
Maxam-Gilbert Sequencing
Differing concentrations of salt are used in four different tubes - A, T, C, G - Usually DMS (dimethylsulphate), FA (formic acid), H (hydrazine), and H+S (hydrazine + salt) --> read on a gel
Coagulopathies
Disorder of blood coag caused by inherited or acquired defects in coag proteins, platelets, or vasculature e.g. Von Willebrand's dz, hemophilia, Factor V Leiden
Sanger sequencing method
Divided into 4 samples (ddA, T, G, C) Label with radioactive/dye oligo at 3' end Mix with taq, dNTPs, ddNTP and incubate run on gel --> frags will terminate at different lengths
What is one way you can increase the yield/quality of DNA/RNA after running gel?
Do an EtOH ppt
Base Excision repair (BER)
Done by DNA glycosylase, AP endonuclease Cleaves glycosidic bond of a single base base, leaving apurinic/apyrimidinc site
Nucleotide Excision repair (NER)
Done by endonucleases Removes a span of nt's by cleaving phosphodiester bond
Graft versus host disease (GVHD)
Donor cells recognize host (recipient) cells as foreign and attack and destroy
What types of probes are used for FISH?
Dual fusion: 2 probes flank the breakpoint at both t locations CEN probes: centromeric probes bind to repetitive alpha satellite sequences Telomeric probes Whole chr paints
Which specimen tubes are the best for use with molecular assay?
EDTA (lavender/purple) ACD (yellow)
Breast cancer, Her1/ErbB1
EGFR, estrogen receptor (ER), is overexpressed Estrogen binds, ER dimerizes -> TXN of genes that promote proliferation Dx: IHC, FISH, qPCR Treatment: Tamoxifen, raloxifene, faslodex
Analyte specific reagent (ASR)
FDA defines analyte specific reagents (ASRs) in 21 CFR 864.4020 as "antibodies, both polyclonal and monoclonal, specific receptor proteins,ligands, nucleic acid sequences, and similar reagents which, through specific binding or chemical reaction with substances in a specimen, are intended to use in a diagnostic application for identification and quantification of an individual chemical substance or ligand in biological specimens.
FDA
FDA is responsible for protecting the public health by assuring the safety, efficacy and security of human and veterinary drugs, biological products, medical devices, our nation's food supply, cosmetics, and products that emit radiation. also responsible for advancing the public health by helping to speed innovations that make medicines more effective, safer, and more affordable and by helping the public get the accurate, science-based information they need to use medicines and foods to maintain and improve their health.
Deoxyribonuclease I
From bovine pancrease, digests ss and dsDNA at pyrimidines. Typically used to remove DNA from RNA preparations.
Prothrombin
G20210A A bleeding disorder that slows the blood clotting process. Mutations in the FII gene cause prothrombin deficiency.
Exons
Gene sequences that represent codons used in TLN to protein
How can you tell if you have good RNA using gel electrophoresis?
Good RNA will have a 2:1 intensity (28S : 18S) if 18S is more, RNA degradation is possible
Major histocompatibility complex (MHC)
Group of genes located on 6p MHC gene products are called human leukocyte antigens (HLA)
What is bDNA used to detect?
HIV Hepatitis
What pathogens can you detect using NASBA?
HIV Hepatitis HTLV CMV
Z-DNA conformation
Left-handed caused by stress or torsion (e.g. during transcription)
Serological Analysis of the MHC
HLA Typing - known anti sera + recipient's lymphocytes Cytotoxicity reading > 6 ( 51 - 80% dead cells), recipient has an Ag matching the panel antibody Screening - recipient Ab + ref lymphocytes % PRA >50% = recipient highly sensitized Cross matching - recipient Ab + donor lymphocytes If donor cells are killed by recipient's sera, it's a positive cross match and donor cannot be used
HLA class I
HLA-A, HLA-B, HLA-C Expressed on all nucleated cells Composed of an α and β-2 chain (Domains:α1, α2, α3) Polymorphisms located on chr 6, exon 2 and 3
HLA class II
HLA-DP, HLA-DQ, HLA-DR Expressed on Ag presenting cells Composed of an α (α1 & α2) and β (β1 & β2) Polymorphisms located on chr 6, exon 2
Which specimen tubes are not good for use with molecular assays?
Heparin (brown/green) inhibits several enzymes used in molecular assays
If fragments are dissolved in 50% formamide will the stringency be higher or lower?
Higher
What are two biological exceptions to positive identification by autosomal STR?
Identical twins and clones have identical nuclear DNA profiles
Aneuploid
Increased number of chr's (eg. Down's syndrome)
Topoisomerase I
Induces ss breaks Remove DNA supercoils during TXN and DNA replication; for strand breakage during recombination; for chr condensation; and to disentangle intertwined DNA during mitosis
How does EtBr cause DNA to fluoresce?
Intercalates into the double helix Absorbs UV ~300 nm, emits ~600 nm
Cleavase/Invader
Invader & signal probe added to target Cleavable substrate is formed if mutation is present Signal probe is cleaved to form invader in the next step FRET probe is added; if invader hybridizes, cleavase cuts flap, separating R and Q
What is the genetic abnormality of: iso(X)(q10)
Isochormosome comprised of the long arms of the X chr
Nucleic Acid Sequence Based Amplification (NASBA)
Isothermal, single tube rxn High sensitivity Enzymatic rxns take place concurrently
Loop-mediated isothermal amplification (LAMP)
Isothermal, single tube technique for the amplification of DNA Uses 4 different primers that recognize 6 regions on target gene Stem-loop structure forms which is used as a template for lamp cycling (SDA)
Sanger Sequencing
Known as deoxy chain terminating sequencing; A primer complementary to the 5' region of DNA is used. The primer is typically labeled with P32 (internal labeling) or a fluorescent dye. Here, modified ddNTPs derivatives are added which lack the OH group found on the 3' carbon of the dNTPs. DNA synthesis will stop upon incorporation of a ddNTP because the bond between the phosphodiester bond cannot be established.
DNA Polymerase δ (Euk)
Lagging strand synthesis DNA repair, exonuclease, replaces primers as it encounters Okazaki fragments
What are some of the benifits of FISH?
Large number of cells may be scored Dual color --> multiple targets Many sample types
DNA Polymerase ε (Euk)
Leading strand synthesis exonuclease
Pyrimidine
One carbon ring Cytosine, Thymine, Uracil
Ligase Chain Reaction (LCR)
Ligation of 2 adjacent primers, which uniquely hyb to one strand of the target Upstream 3' end coincides w/a potential single bp diff in the target sequence If the ends match -> ligated by ligase -> act as a template for the next step 2nd set of primers that are complementary to 1st set -> amplification via pcr probe amp = mutation no probe amp = no mutation
What are the two types of isolation/extraction methods?
Liquid phase (organic & inorganic) Solid phase (Qiagen)
What is the best temperature to store DNA?
Long term = -70C short term = -20C
What is the best temperature to store RNA?
Long term = -70C short term = -20C
If fragments are dissolved in a high concentration of NaCl will the stringency be higher or lower?
Lower
Histone methylation
Lysine (K) and arginine (R) can be methylated Common on K residues of H3 and H4 tails Methylated = silenced Heterochromatin
Histone acetylation and deacetylation
Lysine (K) residue on N-termini Acetylation = active, removes + charge Deacetylation = inactive Euchromatin
Molecular beacons
Measures accumulation of product at the annealing step Contains target specific seq and inverted repeat that forms stem-loop At annealing step probe hyb's to target, separating R and Q
Spectrophotometer
Measures amount of light absorbed Quantitative measurement of [DNA/RNA]
In-vitro diagnostics (IVD)
Medical devices intended to perform diagnoses from assays in a test tube, or more generally in a controlled environment outside a living organism.
Retrotransposons
Mobile genetic elements which can increase genome size and insert itself within coding/noncoding regions
What is the genetic abnormality of: 45, X
Monosomy X, Turner's syndrome
Real-Time PCR/qPCR
PCR based method which is used to amplify and quantify a targeted DNA molecule. Enables both detection and quantification. The quantity can be either an absolute number of copies or a relative amount when noramalized to the DNA input.
Scorpion probes
PCR prod is covalently bound to dye; primer is bound to molc beacon type seq After extension, target specific seq will unfold w/ the newly synthesized target seq, separating R and Q
What are some disadvantages of PCR?
Must know the sequence first Prone to contamination May not be 100% specific Specificity dependent on temp and [Mg]
What are the clinical uses for DNA sequencing?
Mutation detection Confirm mutation by other method Resistance testing HLA genotyping
What is SDA used to detect?
Mycobacterium tuberculosis Chlamydia trachomatis
Should you freeze blood or bone marrow if you are going to use it in a molecular assay?
NO Room temp 22-25C Neutrophils will degranulate if frozen
Pyrosequencing
No gels, fluorescent dyes, sequencing ladder, or ddNTPS; Pyrophosphate (PPi) is released when the phosphodiester bond forms between the dNTP and the primer and is converted to ATP. The ATP then generates a luminescent signal by luciferase-catalysed conversion of luciferin to oxyluciferin. This is repeated with each of the nucleotides - the generation of a signal indicates which nucleotide is the correct base in the sequence. GTTAC (dG peak, dT peak (double that of dG), dA peak, dC peak. Most useful for short to moderate sequencing analysis, or SNPs. Used in HLA
Is 47;XXY a normal karyotype?
No, this is XXY syndrome
Introns
Non-coding sequences that are spliced out before TLN
SyBr green
Non-specific intercalation into the minor groove of dsDNA, can be used in qPCR
How is translation terminated?
Occurs when stop codon enters A site Release factor recognizes stop codon, hydrolyzes ester bond with P site, releasing aa chain
What makes DNA negatively charged?
Phosphate groups of the phosphate:ribose backbone
Irinotecan
Prevents DNA from unwinding by inhibition of topoisomerase 1 Inactivated by glucuronidation to uridine diphosphate glucoronosyltransferase 1A1 (UGT1A1)
What is the use of uracil-N-glycosylase (UNG) in PCR?
Prevents contamination by destroying amplicons containing dUTPs
Poly-A tail
Prevents mRNA from being degraded in cytoplasm 100-250 A's at 3' end
CMS
Previously known as the Health Care Financing Administration (HCFA), is a federal agency within the United States Department of Health and Human Services (DHHS) that administers the Medicare program and works in partnership with state governments to administer Medicaid, the State Children's Health Insurance Program (SCHIP), and health insurance portability standards. In addition to these programs, CMS has other responsibilities, including the administrative simplification standards from the Health Insurance Portability and Accountability Act of 1996 (HIPAA), quality standards in long-term care facilities (more commonly referred to as nursing homes) through its survey and certification process, and clinical laboratory quality standards under the Clinical Laboratory Improvement Amendments.
Qβ replicase
Probe amplification Target (ssDNA/RNA) and to tube w/ reporter probe (has QB reporter Target:reporter hyb to capture probes > complex is hyb to capture probe with magnetic bead > complex is bound to well and washed Target:reporter released > QBpol is added > probe is amplified and detected via colorimetric or flurogenic methods Detects: mycobacteria, Chlamydia, HIV, CMV
Ligase Chain Reaction (LCR)
Probe amplification Two adjacent primers are ligated and amplified by a 2nd set of primers if mutation is present at 3' end of upstream primer Can detect a 1 bp mis-match
Multiplex Ligation-dependent Probe Amplification (MLPA)
Probe amplification; multiple targets amplified in a single rxn 2 oligos: both contain sequence specific probe and universal primer Oligos hybridize adjacent to each other > ligase closes gap > PCR with primers that are specific to universal primer sites on the oligos
DNA Polymerase I (Prok)
Processes Okazaki fragments Replaces RNA primers with DNA (exonuclease activity) Excision repair & proof reading
Feedback inhibition
Product of pathway is noncompetitive inhibitor Binds to allosteric site to slow down rxn b/c too much product
Exonuclease II
Proofreading function of the pol Degrades ssDNA from 3'-->5'
Histones
Proteins that DNA tightly coils around to form chromosomes Octamer, 2 ea of: H2A, H2B, H3, and H4 Histones are hydrophobic (basic K & R,+) DNA is hydrophilic (P backbone, -) +/- interaction keeps them bound
What some indirect analysis methods?
RFLP linkage analysis
RT-PCR
RNA --> cDNA first strand synthesis
The three biochemical activities of reverse transcription
RNA-dependent DNApol, Ribonuclease H, and DNA-dependent DNApol --> all used to create ds cDNA from RNA
Complement-dependent cytotoxicity test (CDC)
Receipient alleles determined by using a panel of Ab against known HLA types Cross-reactive: leukocyte being tested has Ag matching Ab in well
TaqMan
Relies on the 5' exonuclease cleavage activity of Taq pol to cleave a dual labeled probe during hybridization to the complementary target sequence. Only emits a signal once separated from quencher.
Exonuclease III
Removes 5' mono-nt's from the 3' end of the dsDNA in the presence of Mg2+ and Mn2+. Removes nucleotides from blunt ends, recessed ends, and nicks, but NOT overhangs!
Telomeres
Repeat sequence (TTAGGG) at the ends of chr, protect chr from degradation
How does PFGE separate larger fragments more efficiently than standard electrophoresis?
Repeated reorientation forces larger fragments through the gel matrix more efficiently
Endonucleases (Prok)
Restriction enzymes Cleaves phoshpodiester bonds w/i poly-nt chain Recognition site is palindromic sequence Types I-V
What method would you use if you knew the gene sequence and the mutation?
Reverse Dot Blot
A-DNA conformation
Right-handed Deep narrow major groove, wide shallow minor groove Dehydrated DNA takes this form
B-DNA conformation
Right-handed Wide major groove, narrow minor groove Common form found in cells
What does smearing on a gel indicate?
Sample degradation Loaded too much
Name 3 assays by which Factor V Leiden R506Q mutation can be detected:
Sequence specific PCR, PCR-RFLP, Invader Assay
SOLiD Sequencing (NextGen)
Sequencing by ligation. A pool of all possible oligonucleotides of a fixed length are labeled according to the sequenced position. The oligonucleotides are annealed and ligated, the preferential ligation by DNA ligase for matching sequences results in a signal informative of the nucleotide at that position. Before sequencing, the DNA is amplified by emulsion PCR and the resulting beads (each containing single copies of the same DNA) are deposited on the glass slide for sequencing.
Drug metabolism
Several genes are responsible for variances in drug metabolism and response, CYP450 is the most well known CYP metabolism phenotypes: extensive metabolizer (EM), intermediate, ultra-rapid, and poor
Okazaki fragments
Short fragments of DNA synthesized by DNApol δ using the lagging strand (3'->5') as a template
Enhancers
Short regions of DNA that bind proteins (TXN factors) that enhance TXN of a gene
Hybrid capture assays (HCA)
Signal amplification Target DNA is released from the cell, denatured, and binds RNA probe DNA:RNA is recognized and binds Ab on solid support DNA:RNA are detected by adding Abs that bind w/ AP, substrate is added
Branched DNA (bDNA)
Signal amplification Target captured by probes on a solid support Extender, pre-amp, and amp probes hybridized Amp bind alkaline phosphatase Dioxetane is added as a substrate for chemiluminescence Measured with a luminometer
Haploid
Single copy of each chr (humans have 23)
What are primer dimers?
Size is sum of two primers Primers hyb and are extended by Taq
CAP
The College of American Pathologists (CAP), is a medical society serving more than 18,000 physician members and the global laboratory community. It is the world's largest association composed exclusively of board-certified pathologists and pathologists in training and is the worldwide leader in laboratory quality assurance. The College advocates accountable, high-quality, and cost-effective patient care.
Describe the growth of the nucleic acid chain
The chain grows by the attachment of the 5' phosphate group of an incoming nucleotide to the 3' hydroxyl group of the last nucleotide on the growing chain
Pharmocogenomics
The study of genetic factors that influence how a drug works. The goal is to understand how a person's genotype affects an individual's response to drugs. It deals with the influence of genetic variation on drug response in patients by correlating gene expression or snp's with a drug's efficacy or toxicity
Carbemazepine (Tegretol)
Treat bipolar disorder, seizures, neuropathic pain Dangerous/fatel skin rxns w/ HLA alleles: HLA-B*1502 HLA-B58
Gefitinib (Iressa)
Treats EGFR+ (Her1, Her2) breast cancer Tyr kinase antagonist Metabolized by CYP3A4 to its active form
Tamoxifen
Treats ER+ breast cancer ER antagonist Metabolized by CYP2D6 and 3A4 to its active form
Trastuzumab (Herceptin)
Treats Her2/Neu/ErbB2+ (17q12 over expression) breast cancer. mAb binds extracellular domain of EGFR receptors, blocking mitogen binding
What is the genetic abnormality of: 47,XY,+18
Trisomy 18: Edwards Syndrome
A CEN probe is used to visualize chr 21. Three fluorescent signals are observed in the patient's cells when they are stained. These results are consistent with what chr disorder?
Trisomy 21, Down's syndrome
Purine
Two carbon rings Adenine, Guanine
Diploid
Two copies of each chr (humans have 46)
Transcription-Mediated Amplification (TMA)
Two enzymes: RT and RNApol Isothermal RNA or DNA
Human papillomavirus (HPV)
Types 16 and 18 cause most cervical cancers
Stop codons
UAG UAA UGA
Gyrase (topoisomerase II)
Unwinds supercoiling caused by unwinding at the rep fork by introducing DSBs
Melt Curve Analysis
Used for SNPs; Specimens with identical sequences should yield the same peak at the expected Tm and specimens containing different sequences will yield two or more peaks. (FRET Probes - dissociation curves)
Single-Stranded Conformational Polymorphism Ananlysis (SSCP)
Used for known gene, unknown mut Mutation screening Short PCR products form 3D conformation when cooled --> muts have different conformation than WT Non-denaturing PAGE, muts migrate different than WT
Ribosomes
Where TLN occurs Prok: 30s and 50s Euk: 40s and 60s Catalyzes peptide bond between a.a.'s
Gene mutations
affect single genes and are often small changes in the DNA sequence
Strand Displacement Amplification (SDA)
after the initial denaturation step the reaction proceeds at one temperature. Normally used for M. tuberculosis, C.trachomatis, and N. gonorrhoeae.
What can cause primer dimers?
annealing temp too low too much primer
Stringency
conditions of hybridization that control the specificity of binding of the probe to the target sequence
topoisomerase II
cuts both strands of one DNA double helix, passes another unbroken DNA helix through it, and then reanneals the cut strands
Dye terminator
ddNTPs are used and fluorescently labeled instead of the primer. All four reactions are performed in the same tube. Terminated nucleotides are amplified.
Why does Sanger sequencing use ddNTPs instead of dNTPs?
ddNTPs lack of a 3' OH which makes it impossible for pol to add more nucleotides --> chain termination
Methylation of cytosine bases 5' to the gene will increase or decrease expression?
decrease
siRNAs complementary to the gene transcript will increase or decrease expression?
decrease
How can you increase strigency in a hybridization?
decrease [salt] increase [formamide] increase temp
Angelman syndrome
del(15)(q11q13) maternal; paternal is imprinted Ataxia, seizures, inappropriate laughter
Prader-Will syndrome
del(15)(q11q13) paternal; maternal is imprinted Congenital dz, mental retardation, short stature, obesity, hypogonadism
Chronic lymphoid leukemia (CLL)
del(17)(p913) TP53 del(11)(q22) ATM del(13q) long arm clonal b-call malignancy, progressive accumulation of mature lymphocytes Most common leukemia Dx: Flow cytometry; 'basket' or 'smudge' lymphocytes Treatment: chemo., BM transplant
Formamide acts as a __________ in a hybridization.
denaturing agent
Centromeric probes (CEN)
designed to hybridize to the high alpha satellite sequences surrounding centromeres. Region specific to detect aneuploidy of chromosomes
ddNTP
dideoxyribonucleoside triphosphate lack a hydroxyl group (OH) at 2' and 3'
Chaotropic agents
disrupts the structure and denatures the DNA by increasing the entropy and non-covalent forces like hydrogen bonds (ex. chemicals like - sodium iodide, or sodium perchlorate)
Restriction enzymes
endonucleases that recognize specific sequences and break the phosphodiester bond of dsDNA
Diagnostic specificity
likelihood of negatives
Diagnostic sensitivity
likelihood of positives
Reverse transcriptase
enzyme that transcribes RNA to cDNA (lacks introns) RNA --> RNA:DNA --> cDNA (dsDNA)
Denaturing agents
formamide, urea, mercaptoethanol
Type I restriction enzymes
have both nuclease and methylase activity in a single enzyme. Bind to host-specific DNA that contains methylated adenines
Vector
helps carry DNA into cell ie plasmids, virus
What is direct analysis?
identifying a specific gene or mutation that caues disease. gene must be known, might need to know mut
Analytical sensitivity is based on _____ and specificity is based on _______.
limit of detection target specificity
Histone acetylation close to the gene will increase or decrease expression?
increase
What is indirect analysis?
inherited marker near gene associated with disease unknown gene and /or mut
Variant
inherited sequence alterations
Transcription
initiation --> elongation --> termination
cDNA
intron free complementary DNA can be inserted into a plasmid
How does PCR work with methylated DNA?
primers are designed to recognize methylated and unmethylated sense strands at gene promoter the methylated bases inhibit enzyme activity at recognition sites
Does heating a solution from 65C to 75C during hybridization raise or lower stringency?
raises
Type III restriction enzymes
resemble type I enzymes in their ability to methylate and restrict (cut) DNA. - adenine methylation occurs on only one strand.
Colicinogenic factors
resistance to bacteriocins, toxic proteins manufactured by bacteria.
R-factors
resistance transfer factors. Carry antibiotic resistance to common antibiotics.
Line Probe Assay (LiPA)
reverse hybridization assay using sequence-specific oligonucleotide probes (reverse SSOP) multi-parameter testing --> single strip
Open Reading Frame (ORF)
sections of DNA that begin with start codons and end with stop codons DNA: 5' --> 3' transcription: 3' --> 5' DNA --> RNA (promoter) translation: 5' --> 3' mRNA
Primary protein structure
sequence of a chain of amino acids
α thalassemia
α genes on chr 16, two from each parent, wt: αα/αα α thalassemia when 1+ of these genes are affected Severity increases with number of genes affected
β thalassemia
β genes on chr 11, one from each parent, wt: β/β β thalassemia when 1+ of these genes are affected Severity increases with number of genes affected
How is translation initiated?
small rRNA (40S) subunit binds mRNA and scans for start codon (AUG) Met-tRNA is brought to the P site Large rRNA (60S) subunit binds
What are some direct analysis methods?
southern PCR - ASO blot, restriction digest SSCP HA
Mantle cell lymphoma (MCL)
t(11;14)(q13;q32), Cyclin D1;IgH Cyclin D1: needed for cell cycle t causes overexpression of cyclin D1 > clonal expansion of B lymphocytes Dx: FISH, CT/PET scan for high glucose metabolism spots
Acute lymphoblastic leukemia (ALL)
t(12;21) TEL-AML1 fusion t(9;22)(q34;q11) BCR-ABL fusion (Philly chr) Abl is a Tyr kinase; t causes Abl to be constitutively expressed > unregulated lymphoblast proliferation Common in children Dx: karyotyping, IHC, S.blot, RT-PCR, q-PCR Treatment: Imatinib (Gleevec), Tyr kinase inhibitor
Follicular lymphoma
t(14;18), IgH;Bcl-2 WT Bcl2 regulates apoptosis t causes overexpression of Bcl2 > immortal cell (clonal B cell expansion) Most common indolent N.H.L. Dx: PCR w/ primers for MBR/MCR & J regions
Burkitt's lymphoma
t(8;14)(q24;q32), c-myc;IgH t causes c-myc to be constitutively expressed > unregulated proliferation (clonal B cell expansion)
Acute myeloid leukemia (AML) Promyelocytic (APL)
t(8;21) RUNX1/RUNX1T1 Common in adults; myeloblasts 'freeze' in current state (don't differentiate) & proliferates forming a clonal population Dx: Flow cytometry, FISH Treatment: Chemo., BM transplant APL t(15;17) PML;RARα, Promyelocytic leukemia protein;Retinoic acid receptor alpha
Chronic myelogenous leukemias (CMLs)
t(9;22) Abl;Bcr (Philly chr) BCR-ABL constitutively active > activates Jak/Stat; inhibits apoptosis > unregulated proliferation of myeloid cells Clonal expansion of myeloid cells in BM Dx:Karyotype, FISH, RT-PCR Treatment: Imatinib (Gleevec)
aminoacyl tRNA
tRNAs that carry amino acids
What is the purpose of primers in PCR?
to intiate replication
Too many and too few ddNTPs result in:
too many ddNTPS will result in many short sequence reads, too little will result in loss of sequencing data but will give a longer read.
TAE Buffer
tris-acetate w/ EDTA good for DNA recovery good for lrg fragments low buffering capacity increases migration of DNA thru gel
TBE Buffer
tris-borate w/ EDTA good for small DNA fragments high buffering capacity decreases migration thru gel
Heterduplex Analysis (HA)
use for known gene, unknown mutation mutation screening bands on gel --> retarded migration from WT due to seq differences
Branched DNA Technololgy (bDNA)
used for DNA or RNA; short probes are used to capture the target nucleic acid and then to multiple reporter molecules, loading the target nucleic acid with signal.
Type II restriction enzymes
used most frequently in the laboratory - do not have inherent methylation activity in the same molecule as the nuclease activity
Transcription Mediated Technology (TMA)
uses RNase H which degrades RNA from the intermediate hybride so denaturing is no longer required; Isothermal process - negates the requirement for thermal cycling to drive rxns. Targeting RNA allows for the direct detection of RNA viruses (HCV, HIV).
