Steps of PCR in sequence are?

Denature DNA, Anneal Primers, Extend DNA

Denature DNA, Extend DNA, Anneal Primers

Anneal Primers, Extend DNA, Denature DNA

Extend DNA, Anneal Primers, Denature DNA

DNA amplification is done by all, except:

Loop-mediated isothermal amplification (LAMP)

The Takayama test is primarily used for what purpose?

To determine the crystalline structure of a stain.

To identify the species of origin of a stain.

What is the purpose of using a dried blood stain's crust in forensic analysis?

Determination of the blood group

Detection of the species of origin

Determination of secretor status

Characterization of the nature of the stain

What is the most informative test for parental identification?

Assessment of developmental defects

PCR Technology for NEET-PG: High-Yield Forensic Medicine Lessons

PCR: Core Concept - Tiny DNA Xerox

Polymerase Chain Reaction (PCR): An in vitro technique for exponential amplification of specific DNA segments.
Purpose: To generate millions of copies from a minute DNA sample, enabling downstream analysis like STR profiling or sequencing.
Inventor: Kary Mullis (1983).
Core Principle: Utilizes thermal cycling (repeated heating and cooling) with key components:
- DNA template (target DNA)
- Primers (short, specific DNA sequences)
- DNA Polymerase (e.g., Taq polymerase)
- Deoxynucleotide triphosphates (dNTPs)

⭐ Taq polymerase, derived from the thermophilic bacterium Thermus aquaticus, is heat-stable, which is essential for withstanding the high temperatures of the denaturation step in PCR cycles without degrading.

PCR: Key Components - The Reaction Cocktail

DNA Template: Source DNA (genomic, plasmid, cDNA) with target sequence.
Primers (Fwd/Rev): Short, synthetic ssDNA (15-30 bases, commonly 18-25); flank target, initiate synthesis.
DNA Polymerase: Thermostable (e.g., Taq from Thermus aquaticus); withstands high temperatures.

⭐ While Taq polymerase lacks 3'→5' proofreading (error rate 1 in 10,000-100,000 bases), modern PCR often uses high-fidelity polymerases with proofreading capabilities for critical forensic applications.
Deoxynucleotide Triphosphates (dNTPs): dATP, dGTP, dCTP, dTTP; building blocks for new DNA.
Buffer Solution: Maintains optimal pH and ionic strength for polymerase activity.
Magnesium Ions ($Mg^{2+}$): From $MgCl_2$; essential polymerase cofactor, affects annealing. Critical concentration. 📌 Mnemonic: "Delicious Pastries Taste Divine, Bring $Mg^{2+}$!" (DNA, Primers, Taq, dNTPs, Buffer, $Mg^{2+}$)

PCR: The Cycle - Heat, Stick, Extend!

📌 Mnemonic: DAE (Denaturation, Annealing, Extension)

Thermal Cycling Process (variable cycles based on DNA quantity and application):
- Denaturation (Step 1): Heat to 94-98°C (varies by polymerase). Separates dsDNA template into ssDNA.
- Annealing (Step 2): Cool to 50-72°C (primer-dependent). Primers bind to complementary sites on ssDNA.
- Extension (Step 3): 68-72°C (polymerase-optimized). DNA polymerase extends primers, synthesizing new DNA.

⭐ Modern forensic PCR utilizes various DNA polymerases (Taq, Pfu, engineered variants) with optimized thermal profiles for enhanced fidelity and efficiency in challenging forensic samples.

PCR: Variants & Use - Forensic Focus

Multiplex PCR: Simultaneous amplification of multiple DNA loci (e.g., STRs). Foundation of modern DNA profiling; saves sample & time.
Real-Time PCR (qPCR): Quantifies DNA; vital for degraded or low-template samples. Assesses DNA quantity & quality pre-amplification.
Reverse Transcriptase PCR (RT-PCR): Detects RNA (e.g., mRNA for body fluid identification). RNA is first converted to cDNA.
Nested PCR: Increases sensitivity for low-template/degraded DNA using two successive PCR runs with different primer sets.
mtDNA PCR: Targets mitochondrial DNA for highly degraded samples (e.g., hair shafts, old bones) where nuclear DNA is insufficient.

⭐ qPCR is crucial for assessing DNA quantity before STR analysis, preventing issues like allelic dropout or preferential amplification of one allele in a heterozygote.

PCR: Evaluation - Power and Pitfalls

Power (Advantages):
- Extreme sensitivity: amplifies minute (pg) or degraded DNA.
- Rapid (hours), highly specific for target DNA.
- Multiplexing: simultaneous analysis of multiple DNA regions.
Pitfalls (Disadvantages):
- High contamination risk: can lead to false positives.
  
  ⭐ PCR's ability to amplify DNA from a single cell underscores the critical need for stringent anti-contamination measures in forensic settings.
- PCR inhibitors (e.g., heme, indigo dye) can prevent amplification.
- Allelic dropout, especially with Low Copy Number (LCN) DNA.
- Differential amplification and stochastic effects with LCN samples.

High‑Yield Points - ⚡ Biggest Takeaways

PCR (Polymerase Chain Reaction) enables exponential amplification of minute or degraded DNA samples.

Key enzyme: While Taq polymerase remains widely used, modern PCR techniques often employ polymerase blends (Taq with proofreading enzymes like Pfu/Tli) for enhanced accuracy and improved yield of longer products.

Core steps: Denaturation (DNA strand separation), Annealing (primer binding to target DNA), Extension (DNA synthesis by polymerase).

Crucial for STR (Short Tandem Repeat) analysis in modern forensic identification and paternity testing under BSA evidence standards.

Highly sensitive, capable of analyzing trace evidence (e.g., single hair, saliva, minute blood spots) admissible under BSA provisions.

Contamination risk is significant, necessitating stringent laboratory protocols and use of negative controls per BNSS evidence collection procedures.

Multiplex PCR allows simultaneous amplification of multiple DNA targets/loci, improving efficiency in forensic casework.

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PCR Technology