1. DNA Typing Methods RFLP- restriction fragment length polymorphism.
AmpliType®PM+DQA1
DNA sequencing
Mitochondrial DNA typing.
STR- short tandem repeats (PCR based).

2. DNA Typing and Criminal Investigations
1980s- Lynda Mann and Dawn Ashworth.
Richard Buckland- kitchen porter.
Confessed to the second murder.
Scotland Yard.
Semen samples and blood from Buckland taken.
Dr. Alec Jeffreys at Leicester University.
DNA Fingerprinting.
Buckland was not the rapist/murderer!
Voluntary blood submission and DNA testing.
Colin Pitchfork and Ian Kelly- bakery workers.
Kelly bragged about the blood switch.
Colin Pitchfork was arrested and subsequently confessed in 1987.
DNA analysis confirmed match.

3. Restriction Enzymes
An enzyme that cuts DNA at specific internal sites in the nucleotide sequence.
They recognize specific double stranded sequences in DNA.
Recognition sites are 4-8 base pairs (bp) long.
Recognition sites are palindromes.
Arrows indicate cut sites.

4. Restriction Digestion

6. The First Human Genetic Fingerprint

7. Gel Electrophoresis
Technique used to separate DNA on the basis of size (number of base pairs).
DNA samples (mixed with loading dye) are loaded into wells.
Samples are pushed through a gel (agarose or acrylamide) while under the influence of an electrical field.
DNA is negatively charged due to phosphate groups and thus migrates towards the positive electrode (anode).
The larger the DNA, the slower it travels.

10. DQA1

11. DQA1

12. AmpliType®PM+DQA1
DQA1 PM

13. PCR- polymerase chain reaction
Kary Mullis- Nobel Prize in chemistry in 1993.
PCR is used to target and replicate any segment of DNA.
Copy high numbers (1 trillion) of target in 2-3 hours.
A technique that involves repeated cycles of 3 steps:
Denature
Anneal
Extension

14. DNA Amplification with the Polymerase Chain Reaction (PCR)
Separate strands (denature) 5’ 3’
Starting DNA Template 5’ 3’
Add primers (anneal) 5’ 3’
Forward primer
Reverse primer 5’ 3’
Make copies (extend primers)

15. Thermal Cycling Temperatures
94 oC
94 oC
94 oC
94 oC
Single Cycle
72 oC
72 oC
72 oC
Temperature
60 oC
60 oC
60 oC
Time
Typically cycles performed during PCR

16. PCR Components
Taq DNA Polymerase- catalyzes the attachment of the nucleotides to the growing strand of DNA.
DNTPs- deoxynucleotide triphosphates (A,T,G,C).
MgCl2- required to activate Taq Polymerase.
Buffer- salt and pH balanced.
Primers- a single-stranded short chain of nucleotides (10-30 nucleotides in length).
DNA Template
Water

17. PCR Reaction 25 µL reactions Thermocycler
PCR tubes- thin, for rapid heat transfer.
Thermocycler
An instrument that is programmed to repeatedly raise and lower the temperature of a heating block.
Cycling Parameters
94°C for 3 minutes- initial denaturation.
26-40 cycles of the following:
94 °C for 30 seconds.
55 °C for 30 seconds.
72 °C for 60 seconds.
72°C for 5 minutes- final extension.
4°C until processing.

18. PCR Products
PCR products are separated on agarose gel.

19. PCR products can be sequenced

20. ABI 377 DNA Sequencing Machines

25. DNA Separation occurs in minutes...
Capillary Electrophoresis (CE)
Fill with Polymer Solution
Argon Ion Laser
m x 27 cm
5-20 kV - +
Burn capillary window
Inlet (cathode)
Outlet (anode)
DNA Separation occurs in minutes...
Data Acquisition and Analysis

26. Capillary Electrophoresis- AB 310

27. ABI Prism 310 Genetic Analyzer
capillary
Syringe with polymer solution
Injection electrode
Autosampler tray
Outlet buffer
Inlet buffer

28. Close-up of ABI Prism 310 Sample Loading Area
Electrode
Capillary
Sample Vials
Autosampler Tray

30. Capillary System

31. DNA Separation Mechanism+ -
DNA-
Size based separation due to interaction of DNA molecules with entangled polymer strands.
Pumpable polymer can be replaced after each run.
Polymer length and concentration determine the separation characteristics.

32. ABI 3100 Array Detection

33. Fluorescent Dyes Used in 4-Color Detection
JOE (Green)
FAM (Blue) FL
ROX (Red)
CXR
NED
TAMRA (Yellow)

34. Fluorescent Emission Spectra for ABI Dyes
5-FAM
JOE
NED
ROX
ABI 310 Filter Set F
100 80 60
Normalized Fluorescent Intensity 40 20
520
540
560
580
600
620
640
WAVELENGTH (nm)
Laser excitation
(488, nm)

35. Principles of Sample Separation and Detection
Labeled DNA fragments (PCR products)
Capillary or Gel Lane
Size Separation
Sample Detection
CCD Panel
Ar+ LASER (488 nm)
Color
Separation
Detection region
ABI Prism spectrograph
Fluorescence

37. MALDI-TOF Mass Spectrometry

38. Short Tandem Repeats (STRs)
AATG
7 repeats
8 repeats
The repeat region is variable between samples while the flanking regions where primers anneal are conserved.
Homozygote- both alleles are the same length.
Heterozygote- alleles differ in length.

39. Multiplex PCR Multiple PCR reactions are run simultaneously in 1 tube.
Up to 16 reactions.
<1 ng sensitivity.
Different fluorescent dyes used to distinguish STR alleles with overlapping size ranges.

40. Position of Forensic STR Markers on Human Chromosomes
13 CODIS Core STR Loci
CSF1PO
D5S818
D21S11
TH01
TPOX
D13S317
D7S820
D16S539
D18S51
D8S1179
D3S1358
FGA
VWA
AMEL
Sex-typing

41. STR Primers

42. Fluorescent Labeling of STR PCR Products
Dyes are attached to one primer in a pair used to amplify a STR marker.
Dye-labeled oligonucleotide is incorporated into PCR product during multiplex PCR amplification giving a specific color “tag” to each PCR product.

43. AmpFlSTR® Identifiler™
D8S1179
D21S11
D7S820
CSF1PO
D3S1358
TH01
D13S317
D16S539
D2S1338
D19S433
D18S51
TPOX
VWA
AMEL
D5S818
FGA
GS500 LIZ size standard
6FAM (blue)
VIC (green)
NED (yellow)
PET (red)
LIZ (orange)