Midterms practice test

Question 1

If 20% of the nucleotides in an organism
are adenine, predict the percentage of
nucleotides that are guanine.
A. 20%
B. 30%
C. 40%
D. 60%

Answer 1

30%

Question 2

Which of the following is not required for
DNA replication by PCR?
A. Oligonucleotide primers
B. DNA polymerase
C. DNAligase
D. Deoxynucleotides

Answer 2

DNAligase

Question 3

A restriction enzyme recognizes the
sequence, 5’ CTAATAG 3’, and cuts as
indicated. Predict the ends that would
result on the complementary DNA strand.
A. 3’G5’ 3’ATATC5’
B. 3’GA5’ 3’TATC5’
C. 3’GATA5’ 3’TC5’
D. 3’GATAT5’ 3’C 5’

Answer 3

3’GATA5’ 3’TC5’

Question 4

The absorbance of a 1:100 dilution of
isolated dsDNA solution, measured at
260 nm, is 0.062. What is a reasonable
estimate for the dsDNA concentration
of the sample, expressed in ug/mL?
A. 3.1
B. 6.2
C. 310
D. 5000

Answer 4

310

Question 5

In the isolation of RNA, diethylpyrocarbonate (DEPC) is used to
A. Inhibit RNase
B. Lyse the cells
C. Precipitate the DNA
D. Remove buffer salts

Answer 5

Inhibit RNase

Question 6

The technique that makes ssDNA from
an RNA template is called
A. Strand displacement amplification
B. Polymerase chain reaction
C. Ligase chain reaction
D. Reverse transcription

Answer 6

Reverse transcription

Question 7

Purification resins used to isolate DNA
take advantage of the fact that DNA is
A. Double stranded
B. Negatively charged
C. Higher in concentration than RNA
D. Higher molecular weight than RNA

Answer 7

Negatively charged

Question 8

After performance of DNA electrophoresis, the isolated bands in the kilobase size
range appear too close together. Which of
the following can be done with the next
run to improve the appearance/separation
of the bands in the samples?
A. Increase the percent agarose concentration of the matrix
B. Increase the running time of the
electrophoresis assay
C. Increase the sample volume applied
to the gel
D. Decrease the sample volume applied
to the gel

Answer 8

Increase the running time of the
electrophoresis assay

Question 9

Which of the following is commonly used
as a label in molecular tests?
A. Biotin
B. DNase
C. RNase
D. 125I

Answer 9

Biotin

Question 10

Which of the following is not an example
of target amplification?
A. Reverse transcription-PCR (RT-PCR)
B. Transcription mediated amplification
(TMA)
C. Branched chain DNA amplification
(bDNA)
D. Polymerase chain reaction (PCR)

Answer 10

Branched chain DNA amplification
(bDNA)

Question 11

In forensic testing, DNA fingerprinting
can identify individuals with high
accuracy because
A. Human genes are highly conserved
B. Only a small amount of sample is
needed
C. Human gene loci are polymorphic
D. DNA is stable and not easily
contaminated

Answer 11

Human gene loci are polymorphic

Question 12

A 5850-base plasmid possesses EcoRl
restriction enzyme cleavage sites at the
following base pair locations: 36, 1652,
and 2702. Following plasmid digestion,
the sample is electrophoresed in a 2%
agarose gel. A DNA ladder marker,
labeled M in Color Plate 56B, is included
in the first lane, with base pair sizes
indicated in lanes A through D. Which
lane represents the sample pattern that is
most likely the digested plasmid?
A. A
B. B
C. C
D. D

Question 13

Which of the following is characteristic of
DNA chips (i.e., DNA microarrays)?
A. Allow detection and discrimination
of multiple genetic sequences at the
same time.
B. Thousands of oligonucleotide probes
are labeled and placed on glass or
silicon surfaces.
C. Unlabeled target sequences within the
patient sample are detected by
hybridization to labeled probes.
D. All the above

Answer 13

Allow detection and discrimination
of multiple genetic sequences at the
same time.

Question 14

The most useful feature of the molecules
streptavidin and biotin is that they bind
A. Specifically to nucleic acids
B. Only in neutral pH conditions
C. To each other with very high affinity
D. Directly to DNA immobilized on
nitrocellulose

Answer 14

Specifically to nucleic acids

Question 15

What is the theoretic estimation of the
number of DNA target sequences present
(per original double-stranded DNA in
solution) following 15 cycles of PCR?
A. 30
B. 210 (i.e., 1024)
C. 215 (i.e., 32,768)
D. 220 (i.e., 1,048,576)

Answer 15

215 (i.e., 32,768)

Question 16

“Star activity” for a restriction enzyme
refers to
A. An ability to cleave DNA at sequences
different from their defined recognition sites
B. The enzyme’s specificity for sites
of methylation within the nucleotide
sequence
C. The temperature and pH conditions
at which the enzyme will function
optimally
D. The percent increased accuracy of
the enzyme when placed in ideal
conditions of pH

Answer 16

An ability to cleave DNA at sequences
different from their defined recognition sites

Question 17

“Star activity” for a restriction enzyme
refers to
A. An ability to cleave DNA at sequences
different from their defined recognition sites
B. The enzyme’s specificity for sites
of methylation within the nucleotide
sequence
C. The temperature and pH conditions
at which the enzyme will function
optimally
D. The percent increased accuracy of
the enzyme when placed in ideal
conditions of pH

Answer 17

An ability to cleave DNA at sequences
different from their defined recognition sites

Question 18

If a DNA probe is added to nitrocellulose
after the transfer step but before the
blocking step, which of the following will
occur?
A. The probe will nonspecifically bind to
its DNA target.
B. Unoccupied spaces on the nitrocellulose will bind the probe.
C. The DNA target on the nitrocellulose
will be unable to bind the probe.
D. Bound probe will be washed away in
the next wash step.

Question 19

Which of the following items is not used
in the preparation of a DNA probe for
Southern blotting using random hexamer
primers?
A. Template DNA
B. Three unlabeled deoxynucleotides
C. Dideoxynucleotides, with one of them
labeled
D. DNA polymerase

Answer 19

Dideoxynucleotides, with one of them
labeled

Question 20

Which of the following is considered a
“high stringency” condition for DNA
probe protocols?
A. Using wash buffer with highly acidic
pH
B. Washing the matrix with high-salt
buffer
C. Radiolabeling the probe with 35S
rather than 32P
D. Washing the transfer membrane
(e.g., nitrocellulose or nylon) at high
temperature

Answer 20

Washing the transfer membrane
(e.g., nitrocellulose or nylon) at high
temperature

Question 21

When compared to Southern blot
hybridization testing, PCR
A. Is less sensitive to DNA degradation
than Southern blot
B. Includes transfer of DNA onto a nylon
membrane
C. Requires no specialized equipment
D. Is more labor intensive

Answer 21

Is less sensitive to DNA degradation
than Southern blot

Question 22

What enzyme recognizes and cuts
overlapping DNA sequences formed
between mutant or normal probes and
target sequences within samples?
A. Restriction endonuclease
B. DNAligase
C. Cleavase
D. RNaseH

Answer 22

Cleavase

Question 23

Which of the following specimen types is
not used routinely as source material for
molecular genetic tests?
A. Whole blood
B. Buccal scrapings
C. Amniocytes
D. Rectal swabs

Answer 23

Rectal swabs

Question 24

TaqMan probes used to increase specificity of real-time PCR assays generate a
fluorescent signal
A. At the beginning of each cycle during
the denaturation step
B. When the probes bind to the template
(i.e., during annealing)
C. When the probe is digested by 5’ —> 3’
exonuclease activity during extension
of primers (i.e., DNA synthesis)
D. When the reporter fluorophor on the
probe is separated from the quencher
molecule by a restriction enzyme

Answer 24

When the probe is digested by 5’ —> 3’
exonuclease activity during extension
of primers (i.e., DNA synthesis)

Question 25

For the purpose of diagnosing genetic
diseases, what component of whole blood
is used for the extraction of DNA?
A. Leukocytes
B. Plasma
C. Platelets
D. Red blood cells

Answer 25

Leukocytes

Question 26

Which of the following statements best
describes characteristics of RNase?
A. It degrades mRNA but not rRNA.
B. It is found in large concentrations on
hands.
C. Its activity can be eliminated by
autoclaving.
D. Its activity occurs in a limited temperature range between 25 and 65°C.

Answer 26

It is found in large concentrations on
hands.

Question 27

Which of the following is the least likely
inhibitor of PCR?
A. Heme
B. Sodium heparin
C. DEPC (diethylpyrocarbonate)
D. EDTA (ethylenediaminetetraacetic
acid)

Answer 27

EDTA (ethylenediaminetetraacetic
acid)

Question 28

Frequently, DNA probes are used to detect
target sequences in Northern or Southern
blots. Hybridization occurs between DNA
probe and RNA or DNA on the blot,
respectively. To ensure that only exactly
matched complementary sequences have
bound together, the blot is washed under
stringent conditions. Stringency of the
wash steps to remove unbound and
mismatched probe can be increased by
A. High temperature, high NaCl
concentration, and high detergent (i.e.,
SDS) solution
B. High temperature, low NaCl concentration, and high detergent (i.e., SDS)
solution
C. High temperature, high NaCl
concentration, and low detergent (i.e.,
SDS) solution
D. Low temperature, high NaCl concentration, and high detergent (i.e., SDS)
solution

Answer 28

High temperature, low NaCl concentration, and high detergent (i.e., SDS)
solution

Question 29

In RNA, which nucleotide base replaces
thymineofDNA?
A. Adenine
B. Cytosine
C. Guanine
D. Uracil

Answer 29

Uracil

Question 30

The component parts of a dNTP include a
purine or pyrimidine base, a
A. Ribose sugar, and one phosphate
group
B. Deoxyribose sugar, and three
phosphate groups
C. Ribose sugar, and two phosphate
groups
D. Deoxyribose sugar, and two phosphate
groups

Answer 30

Deoxyribose sugar, and three
phosphate groups

Question 31

The component parts of a dNTP include a
purine or pyrimidine base, a
A. Ribose sugar, and one phosphate
group
B. Deoxyribose sugar, and three
phosphate groups
C. Ribose sugar, and two phosphate
groups
D. Deoxyribose sugar, and two phosphate
groups

Answer 31

Deoxyribose sugar, and three
phosphate groups

Question 32

Molecular typing of bacterial strains is
based on restriction fragment length
polymorphisms (RFLPs) produced by
digesting bacterial chromosomal DNA with
restriction endonucleases. Which of the
following techniques is used to separate the
large DNA fragments generated?
A. Ribotyping
B. DNA sequencing
C. Pulsed field gel electrophoresis
D. Reverse transcription-polymerase
chain reaction

Answer 32

Pulsed field gel electrophoresis

Question 33

Which of the following amplification
methods does not employ isothermal
conditions?
A. Nucleic acid sequence-based
amplification (NASBA)
B. Polymerase chain reaction (PCR)
C. Strand displacement amplification
(SDA)
D. Transcription mediated amplification
(TMA)

Answer 33

Polymerase chain reaction (PCR)

Question 34

The coding region of a human gene is called
A. Exon
B. Intron
C. SNP
D. VNTR

Answer 34

Exon

Question 35

The central dogma is that DNA is used to
make RNA, which is then used to make
protein. In this scheme the two processes
that are involved (i.e., DNA to RNA and
RNA to protein) are termed
A. Replication and transcription
B. Synthesis and encryption
C. Transcription and translation
D. Initiation and elongation

Answer 35

Transcription and translation

Question 36

How many chromosomes are contained in
a normal human somatic cell?
A. 22
B. 23
C. 44
D. 46

Answer 36

46

Question 37

An ordered sequence of events makes up
the cell cycle. Which of the following
describes the correct sequence of events
starting at Gl?
A. G1,G2, S,M
B. G1,S,G2,M
C. G1,M,G2, S
D. G1,S,M, G2

Answer 37

G1,S,G2,M

Question 38

Purified DNA remains stable indefinitely
when stored as
A. Small aliquots at 4°C
B. Large aliquots at 25°C
C. Small aliquots at -70°C
D. Large aliquots at -20°C

Answer 38

Small aliquots at -70°C

Question 39

An advantage of amplification technologies for clinical laboratories is that
A. They require inexpensive test reagents
B. They lend themselves to automated
methods
C. Each target molecule sought requires a
unique set of primers
D. Contamination is not a concern when
performing these assays

Answer 39

They lend themselves to automated
methods

Question 40

The assay method that detects the
expression of a gene rather than the mere
presence or structure of a gene is termed
A. RT-PCR
B. TMA
C. Multiplex PCR
D. Ribotyping

Answer 40

RT-PCR

Question 41

Which of the following assays cannot be
accomplished using PCR methods
employing only Tag polymerase?
A. Diagnosis of Chlamydia trachomatis
and Neisseria gonorrhoeae infection
B. Detection of single base pair gene
mutations, such as in cystic fibrosis
C. Detection of HLA-A, B and DR
genotypes
D. Determination of viral load for HCV

Answer 41

Determination of viral load for HCV

Question 42

One method to prevent “false-positive”
PCR results includes the use of dUTP in
the reaction mix, resulting in amplicons
containing U in place of T. The enzyme
used to decrease contamination is
A. Uracil-/V-glycosylase
B. Tag polymerase
C. SI nuclease
D. DNase

Answer 42

Uracil-/V-glycosylase

Question 43

Which double-stranded DNA molecule has the
highest melting temperature?
A. An oligonucleotide with a repeating sequence of
A-A-A at the 5´ end
B. A molecule of 5,000 base pairs with a high
number of A-T base pairs
C. An oligonucleotide with a large number of
repeating C-G-C codons
D. A DNA polymer of 100,000 base pairs

Answer 43

An oligonucleotide with a large number of
repeating C-G-C codons

Question 44

Which base pair sequence is most likely to serve as
a binding site for a restriction endonuclease?
A. A-T-T-C-A
T-A-A-G-T
B. C-T-A-C-T-G
G-A-T-G-A-C
C. C-A-C
G-T-G
D. A-A-G-C-T-T
T-T-C-G-A-A

Answer 44

A-A-G-C-T-T
T-T-C-G-A-A

Question 45

Cloning a human gene into a bacterium in order
to make a large molecular probe requires which
vector?
A. Plasmid
B. Bacterial microsome
C. 30S bacterial ribosome
D. Single-stranded DNA

Answer 45

Plasmid

Question 46

What process can be used to make a DNA probe
produce a fluorescent or chemiluminescent signal?
A. Enzymatic attachment of acridinium esters to
terminal ends of the probe
B. Substitution of biotinylated or fluorescent
nucleotides into the probe
C. Splicing the gene for β-galactosidase into the
probe
D. Heat denaturation of the probe followed by acid
treatment

Answer 46

Substitution of biotinylated or fluorescent
nucleotides into the probe

Question 47

What term describes the products produced when
DNA is digested by restriction endonucleases?
A. Mosaicisms
B. Chimeras
C. Amplicons
D. Restriction fragment length polymorphisms

Answer 47

Restriction fragment length polymorphisms

Question 48

What reagent is most commonly used to stain
DNA separated by electrophoresis?
A. Silver nitrate
B. Nicotinamide adenine dinucleotide
C. Cationic dye
D. Ethidium bromide

Answer 48

Ethidium bromide

Question 49

Which technique is used to detect DNA
containing a specific base sequence by applying a
labeled probe to DNA bands immobilized onto
nitrocellulose paper following electrophoresis?
A. Southern blot
B. Northern blot
C. Dot blot
D. Western blot

Answer 49

Southern blot

Question 50

Which of the following types of mutation causes
the premature termination of protein synthesis?
A. Missense
B. Nonsense
C. Insertion
D. Frame shift

Answer 50

Nonsense

Question 51

In humans, which component of a gene is
translated into a protein?
A. Intron
B. Exon
C. Promoter
D. TATA box

Answer 51

Exon

Question 52

Which statement best describes a DNA
polymorphism?
A. A point mutation arising in a gene
B. Any change in DNA that is associated with
abnormal function
C. A change in the base sequence of DNA that is
translated into an abnormal protein
D. A variation in DNA that occurs with a frequency
of at least 1%

Answer 52

A variation in DNA that occurs with a frequency
of at least 1%

Question 53

Which of the following is the most common type
of polymorphism?
A. Single nucleotide polymorphism (SNP)
B. Variable number tandem repeat (VNTR)
C. Short tandem repeat (STR)
D. Short repetitive interspersed element (SINES)

Answer 53

Single nucleotide polymorphism (SNP)

Question 54

Which of the following mechanisms facilitates
DNA separation by capillary electrophoresis?
A. Molecular sieving
B. Partitioning
C. Adsorption
D. Deflection

Answer 54

Molecular sieving

Question 55

The polymerase chain reaction (PCR) involves
three processes. Select the order in which these
occur.
A. Extension→Annealing→Denaturation
B. Annealing→Denaturation→Extension
C. Denaturation→Annealing→Extension
D. Denaturation→Extension→Annealing

Answer 55

Denaturation→Annealing→Extension

Question 56

In the PCR cycle, how is denaturation
accomplished?
A. Heat
B. Alkali treatment
C. Addition of sulfonylurea
D. Formamide

Answer 56

Heat

Question 57

What is the composition of the primer used
in PCR?
A. A cocktail of enzymes and nucleotide
triphosphates that bind to the target
B. An oligonucleotide complementary to bases at
the 3´ end of the target
C. A small piece of dsDNA that attaches to the
template
D. A probe made of mRNA that binds downstream
from the target

Answer 57

An oligonucleotide complementary to bases at
the 3´ end of the target

Question 58

The master mix solution used for PCR contains
which of the following reagents?
A. Deoxyribonucleotide triphosphates
B. Deoxyribonucleotide monophosphates
C. Deoxyribonucleosides
D. Ribonucleotide monophosphates

Answer 58

Deoxyribonucleotide triphosphates

Question 59

What is the unique characteristic of the DNA
polymerase, Taq DNA polymerase, used in PCR?
A. It can be enzyme labeled
B. It is more efficient than eukaryotic polymerases
C. It is heat stable
D. It works with DNA of any species

Answer 59

it is heat stable

Question 60

In PCR methods, how can several targets be
copied simultaneously and detected?
A. By following the increase in absorbance at
260 nm during melting
B. By labeling multiple primers with specific fluors
C. By substitution of hybridization probes for
primers
D. By analysis of adenosine tail signatures

Answer 60

By labeling multiple primers with specific fluors

Question 61

Which formula predicts the number of PCR
products that can be produced?
A. 2n where n is the number of cycles
B. N4 where N is the number of cycles
C. p2 + 2pq + q2 = 1 where p and q are the number
of primers
D. N2/2 where N is the number of cycles

Answer 61

2n where n is the number of cycles

Question 62

How can PCR be applied to the detection of
human immunodeficiency and other RNA viruses?
A. The virus must be inserted into human DNA by
viral integrase prior to PCR
B. Substitute deoxyuridine triphosphate in place of
deoxythymidine triphosphate in the master mix
C. Add a heat-stable reverse transcriptase enzyme to
the master mix
D. Substitute ribonucleotide triphosphates for
deoxyribonucleotide triphosphates in the
master mix

Answer 62

Add a heat-stable reverse transcriptase enzyme to
the master mix

Question 63

Which statement best describes the method of
branched DNA signal amplification?
A. The DNA template is amplified directly using
patented enzymes
B. Multiple primers are used to create branches of
the template DNA, permitting multiple
extension sites
C. The target DNA is denatured and hybridized to
RNA, and the hybrid molecules are amplified by
both DNA and RNA polymerases
D. The target DNA is bound by multiple
probes, and those are amplified instead of
the target DNA

Answer 63

The target DNA is bound by multiple
probes, and those are amplified instead of
the target DNA

Question 64

A PCR reaction is performed, and the negative
control demonstrates the presence of a detectable
number of PCR products (amplicons) by capillary
electrophoresis. What is the most likely cause?
A. False-positive post-PCR hybridization reaction
due to low stringency
B. Dimerization of PCR primers
C. Contamination of control sample with a trace
amount of template DNA
D. Background signal from gel fluorescence or
inadequate removal of unbound probe

Answer 64

Contamination of control sample with a trace
amount of template DNA

Question 65

How can a false-negative PCR test caused by the
presence of an inhibitor of the reaction in a
patient’s sample be detected?
A. Using a positive control
B. Using an internal control
C. Performing each test in duplicate
D. Performing serial dilutions of the sample

Answer 65

Using an internal control

Question 66

All of the following are requirements for reducing
contamination in DNA amplification methods
except:
A. Use of aerosol barrier pipette tips when
transferring samples or reaction products
B. Preparation of reagents in a dead air box or
biological cabinet
C. A separate area for performing preamplification,
postamplification, and detection steps
D. Pretreatment of samples with high-intensity
ultraviolet light

Answer 66

Pretreatment of samples with high-intensity
ultraviolet light

Question 67

How are PCR methods adapted to yield
quantitative data?
A. By comparing PCR product to an internal
standard
B. By applying a conversion factor to the PCR
signal that converts it to copies per milliliter
C. By determining the mass of PCR product using
ultraviolet spectrophotometry
D. By making serial dilutions of the sample

Answer 67

By comparing PCR product to an internal
standard

Question 68

A PCR analysis of a vaginal sample for Chlamydia
trachomatis gives a negative result (optical density
of biotinylated reaction product below the cutoff
point). The internal control result is also below the
cutoff. Positive and negative controls produced
acceptable results. What action should be taken?
A. The test should be reported as negative
B. The sample should be diluted and the test
repeated
C. The result should not be reported and the sample
should be repeated
D. A preliminary result of negative should be
reported but should be confirmed by further
testing using a different method of analysis

Answer 68

The result should not be reported and the sample
should be repeated

Question 69

In real-time PCR analysis, the absolute
concentration of PCR product is determined
by plotting which two values?
A. Fluorescent intensity versus melting temperature
B. The threshold cycle versus concentration
C. The well factor versus threshold cycle
D. The melting temperature versus concentration

Answer 69

The threshold cycle versus concentration

Question 70

In real-time PCR, quantitation can be done
without standards of known copy number.
Relative quantitation (estimated concentration) is
possible because:
A. Each cycle generates a twofold increase in
product
B. Each cycle threshold represents a 10-fold increase
in product
C. The fluorescence of two samples can be
compared directly
D. Concentration is proportional to fluorescence at
the endpoint of the PCR reaction

Answer 70

Each cycle generates a twofold increase in
product

Question 71

Which real-time PCR parameter can be used to
detect the presence of a contaminant?
A. Threshold cycle
B. Baseline
C. Melting temperature
D. Relative fluorescent intensity

Answer 71

Melting temperature

Question 72

In real-time PCR, what value is needed in order to
determine the threshold?
A. Background signal
B. Melting temperature
C. Maximum fluorescence
D. Threshold cycle

Answer 72

Background signal

Question 73

In real-time PCR, which of the following methods
is not based on using a probe?
A. TaqMan
B. Molecular beacon
C. Scorpion
D. SYBR green

Answer 73

SYBR green

Question 74

Which statement accurately describes the process
of fluorescent in situ hybridization (FISH)?
A. Hybridization is performed on DNA extracted
from cells
B. Hybridization is performed directly on intact
chromosomes
C. Hybridization probes are attached to histones
associated with the chromosomes
D. Hybridization occurs by attachment to the probe
only at the centromere

Answer 74

Hybridization is performed directly on intact
chromosomes

Question 75

Which type of specimen would be unsuitable for
FISH analysis?
A. Paraffin-embedded tissue
B. Cells with chromosomes in metaphase
C. Cells with chromosomes in interphase
D. A cell suspension containing maternal and fetal
blood

Answer 75

A cell suspension containing maternal and fetal
blood

Question 76

FISH can distinguish each of the following
chromosomal abnormalities except:
A. Aneuploidy
B. Translocation
C. Deletion
D. Trinucleotide repeats

Answer 76

Trinucleotide repeats

Question 77

In microarray and macroarray analysis, which
molecules are labeled?
A. The immobilized DNA molecules
B. The sample DNA
C. Both target and sample molecules
D. The substrate matrix

Answer 77

The sample DNA

Question 78

How can all of the mRNA within a sample be
amplified to prepare microarray probes?
A. A specific primer for each mRNA must be
synthesized
B. A primer is made to the polyA tail of mRNA
C. Nonspecific attachment of T7 polymerase occurs
when the cells are treated with detergent
D. Random primer sets are used under low
stringency conditions

Answer 78

A primer is made to the polyA tail of mRNA

Question 79

What is the difference between a microarray and a
macroarray DNA assay?
A. The number of targets is larger on a macroarray
B. The molecular size of each target is larger on a
macroarray
C. The amount of each target is larger on a
macroarray
D. The substrate used for a macroarray is different
from a microarray

Answer 79

he amount of each target is larger on a
macroarray

Question 80

Protein microarray analysis requires the use of
which of the following techniques to generate
protein profile data?
A. Electrophoresis
B. Mass spectroscopy
C. Thin-layer chromatography
D. Gas chromatography

Answer 80

Mass spectroscopy

Question 81

In the reverse transcriptase PCR, the cDNA is synthesized by:
a. reverse transcriptase
b. DNA polymerase
c. Oligo dT primers
d. RNAse H

Answer 81

reverse transcriptase

Question 82

disadvantages of using a nested PCR

Answer 82

susceptible to contamination

Question 83

What is the relationship of the fluorescent dye to the single stranded DNA in every PCR cycle?
a. direct relationship
b. inverse relationship
c. no relationship
d. none of these options

Answer 83

no relationship

Question 84

What will happen to the target DNA sequence if the annealing temperature is too high?
1. No hybridization takes place
2. Primers and templates remains dissociated
3. Production of mismatch hybrids
4. Amplification is more likely to occur at nontarget sites in the template molecule

a. 1 and 2
b. 2 and 3
c. 3 and 4
d. 2 and 4
e. 1 and 4

Answer 84

1 and 2

Question 85

What will happen to the target DNA sequence if the annealing temperature is too low?
1. No hybridization takes place
2. Primers and templates remains dissociated
3. Production of mismatch hybrids
4. Amplification is more likely to occur at nontarget sites in the template molecule

a. 1 and 2
b. 2 and 3
c. 3 and 4
d. 2 and 4
e. 1 and 4

Answer 85

3 and 4

Question 86

What would be the effect to the amplicons, if the denaturation temperature is too low?

Answer 86

the DNA will not completely denature and amplification efficiency will be low

Question 87

Which of the following are correct when using a Multiplex PCR?
1. A minimum of three primer sets designed for amplification of different targets are included in the same PCR reaction.
2. More than one target sequence in a clinical specimen can be amplified in a single tube.
3. The primers used must be selected carefully to have similar annealing temperatures should be complementary to each other.
4. The amplicon sizes should be different enough to form distinct bands when visualized by gel electrophoresis.

a. 1 and 2 b. 1 and 3 c. 2 and 3 d. 2 and 4

Answer 87

2 and 4

Multiplex PCR facts:
More than one target sequence in a clinical specimen can be amplified in a single tube.
The amplicon sizes should be different enough to form distinct bands when visualized by gel electrophoresis.
A minimum of one primer sets designed for amplification of different targets are included in the same PCR reaction.
The primers used must be selected carefully to have similar annealing temperatures but should not be complementary to each other.

Question 88

Which of the following is true about the length of a primer:

Answer 88

If the primers are too short, they might hybridize to nontarget sites and give undesired amplification products

Question 89

Which of the following troubleshooting procedures must be performed when the annealing time is too short?

Answer 89

use an annealing time of at least 30 seconds

Question 90

result if Too few cycles were used

Answer 90

Can lead insufficient
amplification

Question 91

result if Extension time is too short

Answer 91

incomplete
replication of the target

Question 92

result if Annealing times too short

Answer 92

Primers do not have enough
time to bind to the template

Question 93

Annealing temperature was too
high

Answer 93

Primers are unable to bind to the
template

Question 94

Denaturation temperature was
too low

Answer 94

incompletely
denature and amplification
efficiency will be low

Question 95

Denaturation time was too long

Answer 95

DNA might be degraded

Question 96

Denaturation time was too short

Answer 96

incompletely
denature and amplification
efficiency will be low

Question 97

TRUE OR FALSE
To use a more cycles when the temperature concentration was
high and used less cycles when the temperature concentration was low

Answer 97

False; they are inversely proportional

Question 98

TRUE OR FALSE
Rule of thumb (Annealing Temperature)
should be 5 C lower than the melting point of primer

Answer 98

TRUE

Question 99

Implies that data collection and analysis occur in a reaction proceeds

Answer 99

Real Time

Question 100

true or false
Annealing temperature is independent on the primers sequences and is the
critical factor for a successful PCR reaction.

Answer 100

False; it is dependent

Question 101

Statement 1- If the primers are too short, they might hybridize to nontarget sites and give
undesired amplification products.
Statement 2 - Long primers hybridize at a slower rate. The efficiency of
the PCR is therefore reduced if the primers are too long

Answer 101

1 Statement is true, 2 Statement is true

Question 102

Statement 1- If the primers are too short, they might hybridize to nontarget sites and give
undesired amplification products.
Statement 2 - Long primers hybridize at a slower rate. The efficiency of
the PCR is therefore reduced if the primers are too long

A. Neither Statements are correct
B. 1 Statement is true, 2 Statement is true
C. 1 Statement is false, 2 Statement is true
D. 2 Statement is false, 1 Statement is true

Answer 102

1 Statement is true, 2 Statement is true

Question 103

Statement 1:Nested PCR was developed to increase the sensitivity but has a low specificity
of PCR
Statement 2: The products of the first round of amplification are then subjected to a second
round of amplification using the first set of primers

A. Neither Statements are correct
B. 1 Statement is true, 2 Statement is true
C. 1 Statement is false, 2 Statement is true
D. 2 Statement is false, 1 Statement is true

Answer 103

1 Statement is false, 2 Statement is true

rationale: Nested PCR was developed to increase the sensitivity and specificity
of PCR

Question 104

All are true about the multiplex PCR , except

a. more than one target sequence in a clinical specimen
can be amplified in a single tube.
b. The primers used in multiplex reactions must be selected carefully to have
similar annealing temperatures and must be complementary to each
other.
c. The amplicon sizes should be different enough to form distinct bands when
visualized by gel electrophoresis
d. None of the above

Answer 104

The primers used in multiplex reactions must be selected carefully to have
similar annealing temperatures and must be complementary to each
other.

Rationale: must not be complementary to each
other.

Question 105

Statement 1 - A reaction’s Ct is directly linked to the starting concentration of target
sequence
Statement 2 - In the linear part of the PCR amplification, the Ct is directly correlated with
the log of the number of nucleic acid target sequence copies initially present
in the sample

A. Neither Statements are correct
B. 1 Statement is true, 2 Statement is true
C. 1 Statement is false, 2 Statement is true
D. 2 Statement is false, 1 Statement is true

Answer 105

2 Statement is false, 1 Statement is true

rationale: In the linear part of the PCR amplification, the Ct is inversely correlated with
the log of the number of nucleic acid target sequence copies initially present
in the sample

Question 106

Uses two pairs of amplification and two rounds of PCR

a. multiplex PCR
b. RT PCR
c. Nested PCR
d. Digital PCR

Answer 106

Nested PCR

Question 107

Statement 1 - Random hexamers/decamers are 18-base long long single stranded
oligonucleotides of random sequences
Statement 2 - Oligo dT primers are 12-base long single stranded poly dT sequence
that will prime cDNA synthesis from mRNA with poly A tails

A. Neither Statements are correct
B. 1 Statement is true, 2 Statement is true
C. 1 Statement is false, 2 Statement is true
D. 2 Statement is false, 1 Statement is true

Answer 107

Neither Statements are correct

Rationale:
Random hexamers/decamers 6 to 10 long base
Oligo dT primers are 18-base long

Question 108

Primers in RT PCR

Answer 108

Oligo dT and random hexamers/decamers

Question 109

Statement 1: Denaturation: occurs for 20-30 seconds at 94 degrees Celsius.
Statement 2: Annealing: occurs for 20-30 seconds at 50-60 degrees Celsius
Statement 3:Elongation: typically run at 72-74 degrees Celsius for 5 to 15 minutes

A. Neither Statements are correct
B. 1 and 2 Statement is true, 3 Statement is false
C. 1 Statement is false, 2 and 3 Statement is true
D. 2 Statement is false, 1 and 3 Statement is true
E. All statements are true

Answer 109

2 Statement is false, 1 and 3 Statement is true

rationale:Annealing: occurs for 20-40 seconds at 50-60 degrees Celsius

Question 110

True or false
During the elongation step, the DNA polymerase will synthesize new
double stranded DNA.

Answer 110

TRUE

Question 111

Choose A – 1st false 2nd true
Choose B 1st true 2nd false
Choose C both false
Choose D both true

In qPCR, regardless of starting point, all reactions will end at the same, or similar, concentration. qPCR involves gathering of information during the reaction, when different reactions are still in the exponential phase.

Question 112

Choose A – 1st false 2nd true
Choose B 1st true 2nd false
Choose C both false
Choose D both true

Cycle threshold is the number of PCR cycles required to exceed the background fluorescence. It is also the number of which the fluorescence of the given sample crosses the threshold value

Question 113

The conventional PCR can only evaluate the end product of PCR reaction, which can be quantitatively but not qualitatively accurate. The qPCR eliminates the need for post amplification manipulation.

Choose A – 1st false 2nd true
Choose B 1st true 2nd false
Choose C both false
Choose D both true

Question 114

If the denaturation time is too short, the DNA will completely denature and amplification efficiency will be low. For the initial denaturation, use 3 min to activate the polymerase and to denature the template during cycling, use 30 sec.

Choose A – 1st false 2nd true
Choose B 1st true 2nd false
Choose C both false
Choose D both true

Question 115

If the annealing temperature is too high, primers are unable to bind to the template. The rule of thumb is to use an annealing temperature that is 5°C higher than the melting point of the primer.

Choose A – 1st false 2nd true
Choose B 1st true 2nd false
Choose C both false
Choose D both true

Question 116

Which generation of sequencing relied on cycles of the termination of DNA polymerization and recording of the incorporated nucleotides in each cycle?

a. Manual sequencing
b. Third generation sequencing
c. Second generation sequencing
d. None of these
e. First generation sequencing

Question 117

Production of a human protein in bacteria genetic engineering is possible because:
a. Bacterial cell can carry out the RNA splicing reactions
b. The genetic code is universal
c. The mechanism of gene regulation is identical in human and bacteria
d. The human chromosome can replicate in bacterial cell

Question 118

For protein detection, the most commonly used probe is?

Answer 118

Antibody

Question 119

1st statement: Chain-termination DNA sequencing is based on the principle that during DNA synthesis, addition of a nucleotide triphosphate requires a free hydroxyl group on the 3’ carbon of the sugar of the first nucleotide of the growing DNA strand.

2nd statement: However, if a synthetic dideoxynucleotide that lacks a hydroxyl group at the 5’ carbon of the sugar moiety is incorporated at the end of the growing chain, DNA synthesis stops because a phosphodiester bond cannot be formed with the next incoming nucleotide.

a. Only the second statement is true
b. Both statements are true
c. Only the first statement is true
d. Both statements are false

Question 120

A technique of centrifugation that uses repeated centrifugation with a progressive speed that will fractionate the cell homogenates into their components.

Answer 120

differential centrifugation

Question 121

All are the example criteria for selecting a technique for protein quantification and purification, EXCEPT:

Answer 121

Storage temperature

Question 122

the process by which a sample is broken into identical parts so that removing one portion of it does not disrupt and still accurately reflects the remaining sample’s molecular composition.

Answer 122

Homogenization

Question 123

The technique used to detect the presence of DNA or RNA in a Non-fractionated DNA sample is?

Answer 123

Dot Blot Technique

Question 124

Which of the following cell lysis detergent are not example of non-ionic type detergent?
a. Tween 80
b. Triton X-100
c. NP-40
d. Tween 20
e. Sodium dodecyl sulfate

Question 125

Before DNA sequencing, the template DNA must first be prepared by ensuring that there is enough single-stranded version of the DNA to be used. Which among the following is not used to prepare the template DNA?

Answer 125

Phage vector B7

Question 126

The most widely used device to separate a homogenate into different parts or fractions.

Answer 126

Centrifugation

Question 127

The principle techniques to remove contaminants and detergent from proteomic samples use saturated salts to precipitate proteins in the form of ammonium sulfate precipitation or sodium sulfate.

Answer 127

Salting out

Question 128

was the first of the high-throughput DNA sequencing technologies to be made commercially available.

Answer 128

pyrosequencing

Question 129

1st statement: Because the Klenow polymerase has low processivity, it can only synthesize a relatively short DNA strand before dissociating from the template. This limits the length of sequence that can be obtained from a single experiment to about 250 bp.
2nd statement: To improve this short synthesis problem, most sequencing today makes use of a more specialized enzyme, such as Sequenase which is a modified version of the DNA polymerase encoded by bacteriophage T5. Sequenase has high processivity and no exonuclease activity and so is ideal for chain-termination sequencing, enabling sequences of up to 750bp to be obtained in a single experiment.
a. Only the second statement is true
b. Both statements are true
c. Only the first statement is true
d. Both statements are false

Question 130

Which among the following is not a method of how manual sequencing was automated.
a) replacement of radioactive labels by fluorescent labels
b) use of thermal cyclers
c) use of fluorescent detection systems,
d) use of capillary gel electrophoresis
e) none of these

Question 131

Which of the following substances/chemicals will not interfere with the Lowry colorimetric method?

Answer 131

Tris buffer

Question 132

What is the color reaction of Bicinchonic acid assay?

Answer 132

Deep-blue reaction

Question 133

What is the chemical reactant used in Bradford assay?

Answer 133

Deep-blue reaction

Question 134

What is the chemical reactant used in Bradford assay?

Answer 134

Coomassie brilliant blue

Question 135

The principle of this colorimetric assay is based on the complex formation of cupric ions with the proteins.

Answer 135

Biuret reaction

Question 136

This type of buffer for 2DE disrupts the non-covalent and ionic bonds between amino acid residues

Answer 136

Chaotropic agents

Question 137

What is the difference between the Urea-PAGE and SDS-PAGE?

Answer 137

Urea-PAGE Denature RNA strands, while the SDS-PAGE denature proteins and coat with them in negative charges.

Question 138

This device is used for identification of each protein in the sample which undergo digestion, ionization and fragmentation.

Answer 138

Mass spectrometry