Molecular Typing Methods Indian Medical PG Practice Questions and MCQs
Practice Indian Medical PG questions for Molecular Typing Methods. These multiple choice questions (MCQs) cover important concepts and help you prepare for your exams.
Molecular Typing Methods Indian Medical PG Question 1: Which PCR technique is best suited for identifying a syndrome with multiple causative agents?
- A. RT-PCR
- B. Multiplex PCR (Correct Answer)
- C. Nested PCR
- D. Conventional PCR
Molecular Typing Methods Explanation: ***Multiplex PCR***
- **Multiplex PCR** allows for the simultaneous amplification of **multiple DNA targets** in a single reaction, making it ideal for identifying syndromes with numerous potential causative agents.
- This method uses **multiple primer pairs** in one reaction tube, each designed to amplify a specific target sequence, thus efficiently detecting various pathogens or genetic markers.
*RT-PCR*
- **Reverse Transcription PCR (RT-PCR)** is used to detect **RNA targets** by first converting RNA into cDNA, which is then amplified.
- While useful for RNA viruses or gene expression studies, it is not primarily designed for simultaneous detection of multiple diverse causative agents in the same way as multiplex PCR.
*Nested PCR*
- **Nested PCR** uses two sets of primers in sequential reactions to **increase sensitivity and specificity** by reducing non-specific binding.
- This technique is generally employed to detect very low copies of a specific target or to overcome issues with non-specific amplification, rather than for identifying multiple different agents concurrently.
*Conventional PCR*
- **Conventional PCR** amplifies a **single specific DNA target** using one pair of primers per reaction. [1]
- It requires separate reactions for each potential causative agent, making it inefficient and labor-intensive when testing for a syndrome with multiple etiologies.
**References:**
[1] Cross SS. Underwood's Pathology: A Clinical Approach. 6th ed. (Basic Pathology) introduces the student to key general principles of pathology, both as a medical science and as a clinical activity with a vital role in patient care. Part 2 (Disease Mechanisms) provides fundamental knowledge about the cellular and molecular processes involved in diseases, providing the rationale for their treatment. Part 3 (Systematic Pathology) deals in detail with specific diseases, with emphasis on the clinically important aspects., pp. 56-57.
Molecular Typing Methods Indian Medical PG Question 2: Which of the following techniques is primarily used for RNA analysis?
- A. Sanger's technique
- B. Western blot
- C. Next generation sequencing (Correct Answer)
- D. PCR
Molecular Typing Methods Explanation: ***Next generation sequencing***
- **Next-generation sequencing (NGS)**, particularly RNA-Seq, is widely used for **transcriptome analysis** to quantify and discover RNA molecules.
- RNA-Seq allows for the precise measurement of **gene expression levels**, identification of **novel transcripts**, and detection of **splicing variants**.
*Sanger's technique*
- **Sanger sequencing** is primarily used for **DNA sequencing** to determine the exact order of nucleotides in a DNA molecule.
- While it can be applied to cDNA (synthesized from RNA), it is not directly used for **RNA analysis** itself.
*Western blot*
- **Western blot** is a laboratory technique used to detect specific **proteins** in a sample.
- It involves separating proteins by size using gel electrophoresis and then transferring them to a membrane for antibody-based detection, making it unsuitable for direct **RNA analysis**.
*PCR*
- **Polymerase Chain Reaction (PCR)** is used to amplify specific **DNA sequences**.
- While **Reverse Transcription PCR (RT-PCR)** can quantify RNA by first converting it to cDNA, PCR itself does not directly analyze the RNA molecule.
Molecular Typing Methods Indian Medical PG Question 3: PCR is primarily a
- A. DNA sequencing technique
- B. All of these
- C. DNA degradation technique
- D. DNA amplification technique (Correct Answer)
Molecular Typing Methods Explanation: ***Correct: DNA amplification technique***
- **Polymerase Chain Reaction (PCR)** is a laboratory technique used to make millions of copies of a specific DNA segment
- This amplification allows for easier detection, analysis, and manipulation of even very small amounts of DNA
- PCR uses repeated cycles of heating and cooling with DNA polymerase to exponentially amplify target DNA sequences
*Incorrect: DNA sequencing technique*
- **DNA sequencing** determines the exact order of nucleotides within a DNA molecule, which is different from PCR's primary function
- While PCR products can be sequenced afterward, PCR itself does not determine the nucleotide sequence
- Sequencing is a separate technique (e.g., Sanger sequencing, Next-generation sequencing)
*Incorrect: DNA degradation technique*
- **DNA degradation** involves the breakdown of DNA molecules, typically by nucleases or chemical/physical processes
- PCR's purpose is to **synthesize and increase** the amount of DNA, not to break it down
- This is the opposite of what PCR does
*Incorrect: All of these*
- PCR has a specific primary function: **DNA amplification**
- It is not a combination of amplification, sequencing, and degradation techniques
- While PCR can be part of a workflow that includes sequencing, its primary role is amplification only
Molecular Typing Methods Indian Medical PG Question 4: Which of the following is classified as a Category A bioterrorism agent?
- A. Clostridium perfringens
- B. NIPAH virus
- C. Bacillus anthracis (Correct Answer)
- D. Coxiella burnetii
Molecular Typing Methods Explanation: ***Bacillus anthracis***
- **Anthrax**, caused by *Bacillus anthracis*, is a prime example of a Category A bioterrorism agent due to its high mortality, ease of dissemination, and potential for major public health impact.
- Category A agents pose the **greatest threat** to public health and national security.
*Clostridium perfringens*
- *Clostridium perfringens* is classified as a **Category B bioterrorism agent**.
- While it causes **gas gangrene** and food poisoning with moderate severity, it lacks the **high transmissibility** and widespread impact characteristic of Category A agents.
*NIPAH virus*
- **Nipah virus** is classified as a Category C priority pathogen.
- It has the potential for high morbidity and mortality, but its **epidemiological characteristics** (e.g., lower transmissibility than Category A agents) preclude its inclusion in Category A.
*Coxiella burnetii*
- *Coxiella burnetii*, the causative agent of **Q fever**, is classified as a Category B bioterrorism agent.
- Category B agents are moderately easy to disseminate and can cause **moderate morbidity** and low mortality, which is less severe than Category A agents.
Molecular Typing Methods Indian Medical PG Question 5: Restriction fragment length polymorphism is used for:
- A. Detection of gene mutations
- B. Genetic mapping and identification (Correct Answer)
- C. Paternity testing
- D. Forensic analysis
Molecular Typing Methods Explanation: ***Genetic mapping and identification***
- **Restriction fragment length polymorphism (RFLP)** exploits variations in DNA sequences that create or abolish **restriction enzyme recognition sites**, leading to fragments of different lengths.
- These polymorphic fragments serve as **genetic markers** to map genes on chromosomes and identify specific genes or genetic regions.
*Detection of gene mutations*
- While RFLP can detect some mutations by altering restriction sites, it is not the primary or most efficient method for general **gene mutation detection**.
- Techniques like **DNA sequencing** or **PCR-based assays** are typically more sensitive and comprehensive for direct mutation analysis.
*Paternity testing*
- RFLP was historically used for **paternity testing** by comparing inheritance patterns of polymorphic markers between child and alleged father.
- However, it has largely been replaced by more advanced and faster methods like **short tandem repeat (STR) analysis** due to higher discriminatory power and lower DNA requirements.
*Forensic analysis*
- Similar to paternity testing, RFLP was an early technique employed in **forensic analysis** for DNA fingerprinting to identify individuals.
- Modern forensic DNA analysis predominantly uses **STR profiling**, which offers greater resolution, speed, and requires smaller, less degraded samples.
Molecular Typing Methods Indian Medical PG Question 6: An outbreak of staphylococcal infection involving umbilical cords of seven newborn babies was reported in the nursery. Bacteriological survey reveals that two nurses have a large number of Staphylococcus aureus in the nasopharynx. What test should be performed to determine whether these nurses may have been responsible for the outbreak?
- A. Coagulase testing
- B. Nasopharyngeal culture on mannitol salt agar
- C. Bacteriophage typing (Correct Answer)
- D. Protein A typing
Molecular Typing Methods Explanation: ***Bacteriophage typing***
- **Bacteriophage typing** involves using specific **bacteriophages** to identify different strains within a bacterial species based on their susceptibility to lysis by these phages.
- This method helps determine if the specific strain of **Staphylococcus aureus** found in the nurses' nasopharynx matches the strain causing the outbreak in the newborns' umbilical cords, thereby establishing an epidemiological link.
- This is the **classical method** for *S. aureus* strain typing in outbreak investigations. Modern molecular methods like PFGE, MLST, and whole genome sequencing have largely replaced bacteriophage typing, but it remains a fundamental concept tested in medical examinations.
*Coagulase testing*
- **Coagulase testing** differentiates **Staphylococcus aureus** (coagulase-positive) from other coagulase-negative staphylococci.
- While it identifies the species, it does not provide the **strain-level differentiation** needed to link a specific individual to an outbreak.
*Nasopharyngeal culture on mannitol salt agar*
- **Mannitol salt agar** is a selective and differential medium used to isolate and identify **Staphylococcus aureus** from mixed cultures due to its ability to ferment mannitol and tolerate high salt concentrations.
- This test would confirm the presence of **Staphylococcus aureus** in the nasopharynx but would not provide the detailed **strain-specific information** required to trace the source of the outbreak.
*Protein A typing*
- **Protein A** is a common cell wall component of **Staphylococcus aureus** that binds to the Fc region of immunoglobulins.
- While its presence is characteristic of **Staphylococcus aureus**, **Protein A typing** does not offer the necessary **strain-specific resolution** to epidemiologically link an individual carrier to a specific outbreak strain.
Molecular Typing Methods Indian Medical PG Question 7: Western blot is done for:
- A. Protein (Correct Answer)
- B. RNA
- C. Lipid
- D. DNA
Molecular Typing Methods Explanation: ***Protein***
- **Western blot** is a laboratory technique used to detect specific **proteins** in a sample of tissue homogenate or extract.
- It involves separating proteins by **electrophoresis**, transferring them to a membrane, and then detecting them using **antibodies**.
*RNA*
- **Northern blot** is the technique specifically designed for the detection and analysis of **RNA** molecules.
- It involves separating RNA fragments by **electrophoresis**, transferring them to a membrane, and querying with a labeled probe.
*Lipid*
- There is no direct "lipid blot" technique analogous to Western, Northern, or Southern blots.
- **Lipids** are typically analyzed using techniques such as mass spectrometry, thin-layer chromatography, or gas chromatography.
*DNA*
- **Southern blot** is the molecular biology method used for the detection of specific **DNA** sequences in DNA samples.
- It involves fragmenting DNA, separating by **electrophoresis**, and then hybridizing with a labeled DNA probe.
Molecular Typing Methods Indian Medical PG Question 8: What does Polymerase Chain Reaction (PCR) detect?
- A. Antigen
- B. Antibody
- C. Nucleic acid (Correct Answer)
- D. All of the above
Molecular Typing Methods Explanation: **Explanation:**
**Why Nucleic Acid is the Correct Answer:**
Polymerase Chain Reaction (PCR) is a molecular technique used to **amplify specific sequences of DNA**. It utilizes a heat-stable DNA polymerase (like *Taq* polymerase) to create millions of copies of a target genetic sequence. In microbiology, PCR is used to detect the **nucleic acid** (DNA or RNA) of a pathogen. For RNA viruses (like HIV or SARS-CoV-2), a variation called Reverse Transcription-PCR (RT-PCR) is used to first convert RNA into complementary DNA (cDNA) before amplification.
**Why Other Options are Incorrect:**
* **Antigens (Option A):** These are proteins or polysaccharides on the surface of a pathogen. They are detected using immunological assays like **ELISA** (Enzyme-Linked Immunosorbent Assay) or Lateral Flow Assays (Rapid Antigen Tests), not PCR.
* **Antibodies (Option B):** These are host proteins produced by B-cells in response to an infection. They are detected via **Serology** (e.g., ELISA, Western Blot, or Agglutination tests) to identify past or current exposure, whereas PCR identifies the presence of the organism itself.
**High-Yield Clinical Pearls for NEET-PG:**
* **Steps of PCR:** Denaturation (94-96°C) → Annealing (50-65°C) → Extension (72°C).
* **Real-Time PCR (qPCR):** Allows for **quantification** of the microbial load (e.g., Viral Load in Hepatitis C or HIV).
* **Multiplex PCR:** Can detect multiple different pathogens in a single clinical sample simultaneously using different primers.
* **Sensitivity:** PCR is highly sensitive, making it the "Gold Standard" for diagnosing organisms that are difficult to culture (e.g., *M. tuberculosis*, *Chlamydia*, or viral infections).
Molecular Typing Methods Indian Medical PG Question 9: Acridine orange is a fluorescent dye used to bind which cellular components?
- A. DNA and RNA (Correct Answer)
- B. Proteins
- C. Lipids
- D. Carbohydrates
Molecular Typing Methods Explanation: **Explanation:**
**Acridine orange** is a fluorochrome dye that functions as a nucleic acid-selective stain. It has the unique property of **metachromasia**, meaning it can differentiate between double-stranded and single-stranded nucleic acids based on the wavelength of light emitted.
1. **Why A is Correct:** Acridine orange intercalates into **DNA** (double-stranded) and binds electrostatically to **RNA** (single-stranded). When excited by blue light (460 nm) under a fluorescence microscope, DNA-bound dye emits **green fluorescence**, while RNA-bound dye emits **orange-red fluorescence**. This makes it highly effective for detecting microorganisms in clinical specimens (like blood cultures or CSF) where bacteria/fungi appear bright against a dark background.
2. **Why Other Options are Incorrect:**
* **B (Proteins):** Proteins are typically stained with dyes like Coomassie Brilliant Blue or Silver stain.
* **C (Lipids):** Lipids are visualized using lipophilic stains such as Sudan Black or Oil Red O.
* **D (Carbohydrates):** Carbohydrates (glycogen/mucin) are identified using the Periodic Acid-Schiff (PAS) stain.
**High-Yield Clinical Pearls for NEET-PG:**
* **Sensitivity:** Acridine orange is more sensitive than the Gram stain for detecting low concentrations of bacteria (e.g., in buffy coat smears or early positive blood cultures).
* **Rapid Screening:** It is used for rapid screening of malaria parasites (QBC technique) and *Trichomonas vaginalis*.
* **Cell Viability:** It can distinguish between live (green) and dead (red/orange) cells in certain laboratory assays.
Molecular Typing Methods Indian Medical PG Question 10: What is the best technique for initial viral load estimation?
- A. Real-time PCR (Correct Answer)
- B. Widal test
- C. Electrophoresis
- D. Immunofluorescence
Molecular Typing Methods Explanation: **Explanation:**
**Real-time PCR (qPCR)** is the gold standard for viral load estimation because it allows for the **quantification** of nucleic acids in real-time during the amplification process. Unlike traditional PCR, which only provides a qualitative (yes/no) result at the end of the cycle, qPCR uses fluorescent dyes or probes (like TaqMan) to measure the amount of DNA/RNA as it accumulates. The "Cycle Threshold" (Ct) value obtained is inversely proportional to the viral load, making it the most sensitive and accurate method for monitoring diseases like HIV, Hepatitis B, and Hepatitis C.
**Why other options are incorrect:**
* **Widal Test:** This is a serological agglutination test used specifically for diagnosing Enteric (Typhoid) fever by detecting antibodies against *Salmonella typhi*. It cannot quantify viral particles.
* **Electrophoresis:** This technique separates macromolecules (DNA, RNA, or proteins) based on size and charge. While it can visualize genetic material, it is not a primary tool for precise quantification of viral load in a clinical sample.
* **Immunofluorescence (IF):** This technique uses fluorescently labeled antibodies to detect specific viral antigens in cells or tissues. While useful for rapid diagnosis (e.g., Rabies or RSV), it is qualitative or semi-quantitative and lacks the precision required for viral load estimation.
**High-Yield Clinical Pearls for NEET-PG:**
* **Reverse Transcriptase PCR (RT-PCR):** Used for RNA viruses (e.g., HIV, SARS-CoV-2) to convert RNA to cDNA before amplification.
* **Ct Value:** A lower Ct value indicates a **higher** viral load.
* **Viral Load Monitoring:** Essential for assessing the efficacy of Antiretroviral Therapy (ART) in HIV patients; a "detectable" viral load often indicates treatment failure or drug resistance.
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