Nucleic Acid Biochemistry

Question 1

When comparing different species, which of the following best predict the relative number of genes in each species?

a. the size of the organism
b. the complexity of the organism
c. the size of its brain
d. the size of the genome
e. the number of chromosomes

Answer 1

d. the size of the genome.

The number of chromosomes is roughly correlated as well.

Question 2

Chromatin in which of the following states is the most euchromatic?

a. in a Barr body
b. in the centromere
c. in a transcribed gene during G1
d. in a silenced gene during M phase
e. in a sperm nucleus

Answer 2

c. in a transcribed gene during G1

Genes must be euchromatic (decondensed) in order for transcription factors to have access to them. Chromatin is highly condensed during mitosis, when packed in the sperm head, when part of an inactivated X chromosome (Barr body) and in structural, non-expressed regions of a chromosome such as the centromere.

Question 3

Which of the following would be expected for a genetic disease based on a mutation in mitochondrial DNA?

a. it would be more common in men
b. it would be more common in women
c. it would be inherited maternally
d. it would be easy to diagnose based on symptoms
e. it would affect multiple organ systems

Answer 3

c. it would be inherited maternally
e. it would affect multiple organ systems

Mitochondria is maternally inherited but unlike X-linked disorders, will affect both men and women who inherit defective genes. Because of heteroplasmy, different people are affected in different organs and to different extents, making diagnosis tricky. However, since mitochondrial function is essential to so many tissues, symptoms typically arise in multiple organs.

Question 4

Which of the following modifications to histone H3 promote gene silencing?

a. acetylation
b. deacetylation
c. demethylation
d. methylation
e. phosphorylation

Answer 4

b. deacetylation

d. methylation

Question 5

A typical eukaryotic gene consists of which of the following elements?

a. internal ribosome binding sites
b. introns
c. exons
d. enhancers

Answer 5

b. introns
c. exons
d. enhancers

Question 6

Multiple mRNAs can arise from a primary transcript by use of alternative

a. splicing.
b. poly(A) sites.
c. promoters.
d. ribosome binding sites.

Answer 6

a. splicing.
b. poly(A) sites.
c. promoters.

Question 7

Which of the following is (are) encoded by multiple genes present in the human genome?

a. ribosomal RNA
b. transfer RNA
c. histone
d. lysozyme

Answer 7

a. ribosomal RNA
b. transfer RNA
c. histone

Question 8

Which of the following statements is (are) true of the human genome?

a. 1.5 percent of the genome corresponds to protein coding sequences.
b. The median length of an intron is 10 kb.
c. 10 percent of the genome is transcribed into pre mRNA precursors.
d. Most human exons contain 500–1000 base pairs.

Answer 8

a. 1.5 percent of the genome corresponds to protein coding sequences.

Question 9

DNA fingerprinting is a technique based on differences in the

a. length of introns.
b. number of tandem copies of a simple sequence repeat.
c. number of tandem ribosomal RNA genes.
d. size of protein coding genes.

Answer 9

b. number of tandem copies of a simple sequence repeat.

Question 10

Transposition by a bacterial insertion element

a. occurs at a frequency of approximately 1 in 103 cells per generation.
b. can inactivate an essential gene.
c. is mediated through a RNA intermediate.
d. requires the enzyme transposase.

Answer 10

b. can inactivate an essential gene.

d. requires the enzyme transposase.

Question 11

Transposition by a retrotransposon requires activity of which of the following enzymes?

a. RNA polymerase
b. reverse transcriptase
c. DNA methylase
d. DNA polymerase

Answer 11

a. RNA polymerase

b. reverse transcriptase

Question 12

LINES (long interspersed elements)

a. are retrotransposons that lack LTRs.
b. are approximately 300 base pairs long.
c. are a rare class of mobile elements in mammals.
d. use the enzyme transposase for transposition.

Answer 12

a. are retrotransposons that lack LTRs.

Question 13

Human mitochondrial DNA

a. uses the standard genetic code.
b. encodes its own ribosomal RNAs.
c. contains introns like nuclear genes.
d. is larger than yeast mitochondrial DNA.

Answer 13

b. encodes its own ribosomal RNAs.

Question 14

Plant mitochondrial DNA

a. is the same size as human mitochondrial DNA.
b. encodes a 5S mitochondrial rRNA.
c. contains multiple copies that recombine with each other.
d. uses the standard genetic code.

Answer 14

b. encodes a 5S mitochondrial rRNA.
c. contains multiple copies that recombine with each other.
d. uses the standard genetic code.

Question 15

An open reading frame (ORF) is defined as a DNA sequence that

a. begins with a start codon.
b. ends with a stop codon.
c. contains 50 codons.
d. contains approximately an equal frequency of A, T, G, and C.

Answer 15

a. begins with a start codon.

b. ends with a stop codon.

Question 16

Two related genes that are derived from a gene duplication event are considered to be

a. homologous.
b. paralogous.
c. orthologous.
d. members of a gene family.

Answer 16

a. homologous.
b. paralogous.
d. members of a gene family.

Question 17

A transcriptionally active gene compared with a transcriptionally inactive gene would be expected to

a. contain acetylated histones.
b. contain unacetylated histones.
c. be sensitive to DNase I.
d. be resistant to DNase I.

Answer 17

a. contain acetylated histones.

c. be sensitive to DNase I.

Question 18

Scaffold-associated regions

a. are the chromosome attachment points for the mitotic spindle.
b. can insulate transcription units from each other.
c. are the points at which DNA interacts with histone proteins.
d. are found between transcription units.

Answer 18

b. can insulate transcription units from each other.

d. are found between transcription units.

Question 19

Metaphase chromosomes can be identified

a. by shape.
b. by the size and number of introns.
c. by banding patterns with Giemsa reagent.
d. by chromosome painting.

Answer 19

a. by shape.
c. by banding patterns with Giemsa reagent.
d. by chromosome painting.

Question 20

Telomerase

a. extends DNA strands during DNA synthesis.
b. has reverse transcriptase activity.
c. is a protein-RNA complex.
d. replicates repetitious DNA located at the centromere.

Answer 20

b. has reverse transcriptase activity.

c. is a protein-RNA complex.

Question 21

Compare and contrast simple transcription units and complex transcription units.

Answer 21

A simple transcription unit produces a single monocistronic mRNA, which is translated into a single protein. A complex transcription unit produces primary transcripts that can be processed in alternative ways and translated into multiple proteins.

Question 22

Describe the three different ways that multiple mRNAs can arise from a complex transcription unit in eukaryotes.

Answer 22

A complex transcription unit is transcribed into multiple mRNAs by using alternative promoters, poly(A) sites, and splicing. The use of alternative promoters produces mRNAs with different 5´ exons but common 3´ exons. The use of alternative poly(A) sites produces mRNAs with common 5´ exons but different 3´ exons. The use of alternative splice sites produces mRNAs with common 5´ and 3´ exons but different combinations of internal exons.

Question 23

Describe the general organization of the human genome in terms of protein-coding and functional RNA genes, repetitious DNA, and spacer DNA.

Answer 23

The human genome consists of protein-coding and functional RNA genes, repetitious DNA, and spacer DNA. Protein-coding genes and functional RNA genes make up approximately 30 percent of the genome. Protein-coding genes can exist as solitary genes or duplicated genes. Functional RNAs such as tRNA, rRNA, and snRNA are present as tandemly repeated genes. Repetitious DNA makes up almost half of the human genome and is usually concentrated at specific chromosomal locations, e.g., at the centromere. The remainder of the genome consists of spacer or intergenic DNA.

Question 24

Describe the molecular basis for the DNA fingerprinting technique. How can this be used to differentiate between two individuals?

Answer 24

The DNA fingerprinting technique is based on differences in the length of simple-sequence DNAs. Simple-sequence DNA usually occurs in tandem arrays. The number of simple-sequence repeat units at a given genetic locus varies between individuals, and thus the total length of the tandem array differs. These differences in the length of tandem arrays throughout the genome are unique to an individual and is the basis for an individual’s unique DNA fingerprint.

Question 25

Describe the structural features of bacterial insertion sequences and transposons.

Answer 25

Bacterial insertion sequences (IS) are about 1–2 kilobases long. At each end of the IS element is an approximately 50-base-pair inverted repeat. Between the inverted repeats is a region that encodes the enzyme transposase—which is required for transposition or the “cut and paste” operation of the element—to a new site in the genome.

Question 26

Describe the possible role that mobile DNA elements played in evolution.

Answer 26

Mobile DNA elements are hypothesized to have had a profound effect on the evolution of organisms. Insertion of a mobile DNA element into or near a gene can cause a mutation in the gene. Some evidence suggests that recombination between repeat sequences (e.g., mobile elements) of two separate genes can generate a novel combination of exons, a process known as exon shuffling. Unequal crossing over between repeat sequences can result in gene duplication. Furthermore, transposition of DNA adjacent to mobile DNA elements can move transcriptional control elements to new regions of the genome.

Question 27

How does plant mitochondrial DNA differ from mammalian mitochondrial DNA?

Answer 27

Plant mitochondrial and animal mitochondrial DNA are circular molecules that encode for tRNA, rRNA, and essential mitochondrial proteins. In contrast to mammals, plants contain multiple mitochondrial DNAs that appear to recombine with one another. Plant mitochondrial DNAs are much larger and more variable in size than those of other organisms. Plant mitochondrial DNA also encode a 5S mitochondrial rRNA, which is present only in plant mitochondrial ribosomes, and the α subunit of the F1 ATPase. Furthermore, plant mitochondrial DNA uses the standard genetic code, whereas mammalian mitochondria use a modified code.

Question 28

What is a BLAST search and how can it be used to help determine the function of an unknown cloned gene?

Answer 28

The BLAST (basic local alignment and search tool) program searches the DNA/protein databases for significant matches between a query sequence and stored sequences. The search program then assigns a score based on the extent of the match. For an unknown cloned gene, the DNA sequence or predicted amino acid sequence can be used as the query sequence for the BLAST search. If a known gene or protein in the database shows significant similarity to the query sequence, then it is likely that the unknown cloned gene is functionally similar to the known gene.

Question 29

What are the applications of DNA microarrays?

Answer 29

A DNA microarray consists of thousands of individual, closely packed, gene-specific sequences attached to a surface such as glass or a nylon membrane. The power of the microarray is its ability to examine the expression of thousands of genes simultaneously. It is the functional equivalent of performing thousands of Northern blots at one time.

Question 30

Describe the role that nonhistone proteins play in organizing chromosome structure.

Answer 30

Nonhistone proteins provide a structural scaffold for organizing chromatin loops. The chromosome scaffold, which has the shape of a metaphase chromosome, consists of nonhistone proteins that serve as binding sites for chromatin loops.

Question 31

How does chromatin differ between transcriptionally inactive and transcriptionally active regions of DNA?

Answer 31

Experimental evidence indicates that transcriptionally inactive DNA has a condensed chromatin structure. This structure makes the DNA inaccessible to RNA polymerase. In contrast, actively transcribed DNA is present in a more extended, “beads-on-a-string” form of chromatin. DNA with this more open conformation is more accessible to RNA polymerase and other proteins required for transcription.

Question 32

What three functional elements are required for replication and stabilization of chromosomes?

Answer 32

Eukaryotic chromosomes require origins of replication to initiate DNA replication, a centromere for proper segregation of chromosomes during mitosis, and telomeres to stabilize the ends.

Question 33

How many base pairs make up the human genome?
A. 3.3 million
B. 5.1 billion
C. 3.3 billion
D. 5.1 million

Answer 33

C. 3.3 billion

Question 34

When was Sanger sequencing developed and what is another name for it?

Answer 34

1975, chain terminator

Question 35

What is the typical read length for a Sanger sequencing product?
A. 300-800 bps
B. 500-1,000 bps
C. 100-300 bps

Answer 35

A. 300-800 bps

Question 36

What are the major differences between Sanger sequencing and massively parallel sequencing?

Answer 36

1. Longer read length with Sanger
2. Single template read for Sanger, many template reads with MPS
3. Sanger cannot be used for gene expression or quantitative assays
4. No prior knowledge of the genome is required for MPS

Question 37

Which of the following mutations can result in a reduction of β-galactosidase?

a. a mutation in adenylate cyclase
b. a mutation in catabolite activator protein (CAP)
c. a mutation in the CAP site in the lac control region
d. a mutation in the repressor binding site in the operator

Answer 37

a. a mutation in adenylate cyclase

Question 38

Specific DNA control elements in promoters can

a. interact with general transcription factors.
b. interact with repressor proteins.
c. interact with activator proteins.
d. remain unavailable because of condensed chromatin.

Answer 38

a. interact with general transcription factors.b. interact with repressor proteins.c. interact with activator proteins.d. remain unavailable because of condensed chromatin.

Question 39

Reporter genes are used to

a. express enzymes that are not easily assayed in cell extracts.
b. express enzymes that are easily assayed in cell extracts.
c. characterize DNA control elements.
d. characterize reporter plasmids.

Answer 39

b. express enzymes that are easily assayed in cell extracts.c. characterize DNA control elements.

Question 40

The three eukaryotic RNA polymerases can be distinguished by

a. the types of genes they transcribe.
b. the number and types of large subunits.
c. their differential sensitivities to cycloheximide.
d. their differential sensitivities to α-amanitin

Answer 40

a. the types of genes they transcribe.andd. their differential sensitivities to α-amanitin.

Question 41

“Which of the following can be identified using a series of promoter linker scanning mutations?

a. areas of the promoter that are non-essential
b. areas of the promoter that are essential
c. the presence of separate transcriptional control regions

Answer 41

a. areas of the promoter that are non-essentialb. areas of the promoter that are essentialc. the presence of separate transcriptional control regions

Question 42

An enhancer

a. can be located upstream of a promoter.
b. can be located downstream of a promoter.
c. can be located a variable distance from the promoter.
d. is always located within 1 kb of the promoter.
e. can be cell-type-specific.

Answer 42

a. can be located upstream of a promoter.b. can be located downstream of a promoter.c. can be located a variable distance from the promoter.e. can be cell-type-specific.

Question 43

The fact that a specific protein leaves a footprint on a DNA molecule is indicative of

a. a lack of interaction between the specific protein and DNA.
b. protection from DNAse by the specific protein.
c. binding of the specific protein to all types of DNA.
d. binding of the specific protein to a specific sequence of DNA.

Answer 43

b. protection from DNAse by the specific proteinandd. binding of the specific protein to a specific sequence of DNA.

Question 44

The C-terminal activation domain of transcriptional activators is capable of

a. binding to DNA.
b. stimulating transcription.
c. interaction with other transcriptional machinery.
d. functioning in a fusion with a DNA-binding domain from an unrelated transcriptional activator.

Answer 44

a. binding to DNA.
b. stimulating transcription.
c. interaction with other transcriptional machinery.
d. functioning in a fusion with a DNA-binding domain from an unrelated transcriptional activator.

Question 45

Which of the following are not found in DNA-binding proteins?

a. homeodomains
b. zinc fingers
c. leucine zippers
d. CpG islands

Answer 45

d. CpG islands

Question 46

Transcription factors can:

a. exhibit cooperative binding.
b. exist as heterodimers.
c. act to repress transcription of transcription factor genes.
d. undergo conformational changes which alter activity.
e. never interact with co-repressors.

Answer 46

a. exhibit cooperative binding.
b. exist as heterodimers.
c. act to repress transcription of transcription factor genes.
d. undergo conformational changes which alter activity.

Question 47

Which is the first factor to bind at the promoter of eukaryotic genes?

a. RNA polymerase
b. TFIIA
c. TFIIB
d. TFIID
e. TATA box binding protein

Answer 47

d. TFIID,

e. TATA box binding protein

Question 48

Which of the following occur(s) during Pol II transcription preinitiation complex formation?

a. TFIIA binds to TFIIB.
b. TFIIB unwinds the DNA.
c. TFIIB contacts both TATA box binding factor and DNA.
d. DNA bends.

Answer 48

c. TFIIB contacts both TATA box binding factor and DNA.

d. DNA bends.

Question 49

Chromatin-mediated repression of transcription involves

a. modification of lysine residues in histones.
b. large, multiprotein complexes.
c. acetylation of histone tails.
d. deacetylation of histone tails.

Answer 49

a. modification of lysine residues in histones.
b. large, multiprotein complexes.
c. acetylation of histone tails.

Question 50

Which of the following does (do) not require a DNA helicase activity?

a. SWI/SNF function
b. Pol II open-complex formation
c. transcription-factor binding to DNA
d. deacetylation of histone tails

Answer 50

c. transcription-factor binding to DNA

d. deacetylation of histone tails

Question 51

The yeast two-hybrid system can be used to identify

a. proteins that interact with a known or unknown protein.
b. proteins that interact with a kinase domain.
c. cDNAs that encode interacting proteins.
d. co-activators and co-repressors.

Answer 51

a. proteins that interact with a known or unknown protein.
c. cDNAs that encode interacting proteins.
d. co-activators and co-repressors.

Question 52

The expression of which gene(s) is (are) regulated by promoter proximal pausing?

a. hsp70
b. lac operon
c. tat
d. none of the above

Answer 52

a. hsp70

Question 53

The promoter sequences of RNA polymerase III-transcribed genes are located

a. within the transcribed sequences of genes.
b. upstream of the transcribed sequences of genes.
c. downstream of the transcribed sequences of genes.
d. within the first intron.

Answer 53

a. within the transcribed sequences of genes.

Question 54

Regulation of the lac operon is under both negative and positive control. Describe how these two transcriptional control mechanisms regulate expression of the lac operon in the presence of glucose and/or lactose.

Answer 54

In the presence of glucose and the absence of lactose, cAMP levels are low. The lac repressor is bound to the lac operator, which blocks the synthesis of lac mRNA. In the presence of glucose and lactose, the lac repressor is bound to lactose and is unable to bind to the lac operator. However, because cAMP is low in the presence of glucose, very little lac mRNA is synthesized. In the absence of glucose and the presence of lactose, the lac repressor is again unable to bind to the lac operator because it is bound to lactose. However, cAMP levels are high in the absence of glucose. A cAMP-CAP complex forms, which binds to the CAP site and stimulates transcription of lac mRNA.

Question 55

Compare the structure and function of the three eukaryotic RNA polymerases.

Answer 55

In eukaryotic cells, three different RNA polymerases catalyze the formation of different RNAs. RNA polymerase I is located in the nucleolus and synthesizes pre-ribosomal RNA (the precursor to 28S, 5.8S, and 18S rRNAs). RNA polymerase II synthesizes messenger RNAs. RNA polymerase III synthesizes tRNAs, 5S rRNAs, and a number of small RNAs. These small RNAs include an RNA involved in RNA splicing and the 7S RNA of the signal-recognition particle. All three RNA polymerases contain two large sub-units and 15 smaller subunits. Some of these subunits are shared among the different polymerases and others are unique.

Question 56

Describe the three types of eukaryotic promoters.

Answer 56

1. contains a highly conserved sequence located approximately 25-35 base pairs upstream of the transcription start site known as the TATA box. The TATA box acts similarly to a prokaryotic promoter to position RNA polyeramerase II for transcription initiation.
2. lack a TATA box and instead contain an alternative promoter element called an initiator. The initiator sequence is not highly conserved.
3. contains neither a TATA box nor an initiator element. These genes contain a CG-rich stretch of 20-50 nucleotides (CpG islands) approximately 100 base pairs upstream of the start site.

Question 57

How can linker scanning mutation analysis be used to map the location of transcription-control elements?

Answer 57

In linker scanning mutation analysis, a region of DNA that contains putative regulatory elements is cloned into a plasmid upstream of a reporter gene. A series of overlapping linker scanning mutations are introduced into the DNA containing the regulatory elements. The mutations are introduced by scrambling the nucleotide sequence in a short stretch of DNA. The effects of these mutations are evaluated by assaying reporter gene expression.

Question 58

Describe the sequence of events that occurs during formation of a transcription initiation complex on a TATA-box promoter.

Answer 58

A number of sequential protein binding steps occurs during the formation of a transcription initiation complex. The TATA box-binding protein (TBP) included within TFIID first binds to a TATA box in the promoter. Once TBP has bound to the TATA box, TFIIB can bind. The next step is the binding of a pre-formed TFIIF and PolII complex. Then TFIIE and TFIIH bind, completing assembly of the transcription initiation complex.

Question 59

Describe transcription initiation for RNA polymerase I and III transcribed genes.

Answer 59

Transcription initiation by RNA polymerase I is mediated by a core element, which includes the start site of the pre-rRNA gene and an upstream control element, located approximately 100 base pairs upstream. Two transcription factors up-stream binding factor (UBF) and selectivity factor 1 (SL1) bind to and help stabilize the initiation complex. Transcription initiation by RNA polymerase III is mediated by internal promoter elements, termed the A box and B box, present in all tRNA genes. Two transcription factors, TFIIIC and TFIIIB, are required for transcription initiation of tRNA genes. An additional factor (TFIIIA) is required for transcription initiation of 5S rRNA genes.

Question 60

Regulation of the cell cycle is controlled by:

a. telomerase
b. protein kinases
c. ATP
d. growth factors

Answer 60

b. protein kinases

Question 61

What is the function of DNA in the cell?

Answer 61

DNA is a storage system. The function of DNA is to store genetic information.

Question 62

Compare the structure of nitrogen bases. How do purines and pyrimidines differ?

Answer 62

Purines have a double ring, while pyrimidines have a single ring.

Question 63

Write the complementary sequence to the following:

5’ AGG TCA CGT CTA GCT AGC TAG A ‘3

Answer 63

5’ T CTA GCT AGC TAG ACG TGA CCT ‘3

Question 64

Which of the ribose carbons participate in the phosphodiester bond?

Answer 64

The 5’ ribose carbon carries the phosphate group that forms a phosphodiester bond with the hydroxyl group on the 3’ ribose carbon.

Question 65

Which of the ribose carbons carries the nitrogen base?

Answer 65

The 1’ carbon of the ribose carries the nitrogen base.

Question 66

Why does DNA polymerase require primase activity?

Answer 66

DNA polymerase cannot begin synthesis with a 3’ OH group.

Question 67

What is the covalent bond between nucleotides catalyzed by DNA polymerase?

Answer 67

The covalent bond between nucleotides is a phosphodiester bond.

Question 68

Is DNA replication conservative or semi-conservative?

Answer 68

DNA replication is semi-conservative.

Question 69

What is the lagging strand in DNA synthesis?

Answer 69

During DNA replication, the lagging strand is the strand positions 5’ to 3’ with respect to the direction of synthesis, requiring the replication assembly to jump ahead and read 3’ to 5’ back toward the moving replication fork. The leading strand is read continuously 3’ to 5’. Synthesis thus proceeds 5’ to 3’ on both strands.

Question 70

Short pieces of DNA involved in DNA synthesis in replicating cells are called what type of fragments?

Answer 70

Short pieces of DNA involved in DNA synthesis in replicating cells are called Okazaki fragments.

Question 71

Name the function of the following enzyme: polymerase

Answer 71

Polymerase catalyze formation of a phosphodiester bond between nucleotides.

Question 72

Name the function of the following enzyme: helicase.

Answer 72

helicase unwinds nucleic acids, relieving stress on the double helix by breaking and re-attaching phosphodiester bonds.

Question 73

Name the function of the following enzyme: primase

Answer 73

Primase is an RNA polymerase that starts replication in the absence of a 3’ OH group.

Question 74

Name the function of the following enzyme: exonuclease

Answer 74

Exonuclease digests phosphodiester bonds from the ends of nucleic acid molecules.

Question 75

Name the function of the following enzyme: endonuclease

Answer 75

Endonuclease breaks the phosphodiester bonds in the nucleic acids within the polymer chains, rather than from the ends.

Question 76

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. How many HpaII sites are present in this plasmid?

Answer 76

There are three HpaII sites in this plasmid.

Question 77

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. What are the distances between each site?

Answer 77

The distances between the sites are 100, 230, and 500 bp.

Question 78

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. What is the size of the plasmid?

Answer 78

The plasmid is 100 + 230 + 500 = 830 bp.

Question 79

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. A second cut of the plasmid with BamHi yields two pieces, 80 and x bp. How many BamHI sites are in the plasmid?

Answer 79

There are two BamHI sites in the plasmid.

Question 80

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. A second cut of the plasmid with BamHi yields two pieces, 80 and x bp. What is the length of x in base pairs (bp)?

Answer 80

x = 830 - 80 = 750 bp

Question 81

A plasmid was digested with the enzyme HpaII. On agarose gel electrophoresis, you observe three bands: 100, 230, and 500 bp. A second cut of the plasmid with BamHi yields two pieces of 80 and 750 bp. How would you determine where the BamHI sites are in relation to the HpaII sites?

Answer 81

Cut the plasmid with both the BamHi and HpaII restriction enzymes in the same reaction and note the fragment sizes that are produced.

Question 82

A plasmid has one EcoR1 site into which you want to clone a blunt-ended fragment. What type of enzyme could turn an EcoR1 sticky end into a blunt end?

Answer 82

A single-strand exonuclease can digest the EcoR1 overhang, forming a blunt end. Alternatively, a polymerase could fill in the overhang to make a blunt end.

Question 83

Compare how DNA moves from one cell to another by: conjugation.

Answer 83

For conjugation, DNA moves from cell to cell through physical contact.

Question 84

Compare how DNA moves from one cell to another by: transduction.

Answer 84

DNA moves from cell to cell through intermediary viruses or bacteriophages in transduction.

Question 85

Compare how DNA moves from one cell to another by: transformation

Answer 85

In transformation, unprotected DNA moves from cell to cell without physical contact or viral carriers.

Question 86

Bacteria with phenotype A+ are mixed with bacteria with phenotype A- in a culture. Some of the A- bacteria become A+. When A+ bacteria are removed from the culture and A- bacteria are grown in the A+ cell culture medium only, they all remain A-. What type of transfer occurred in the mixed culture?

Answer 86

Conjugation occurred in the mixed culture. If the A-bacteria became positive through transformation or transduction, the cell culture medium from the A+ bacteria would contain DNA or phage, respectively, capable of transforming A- bacteria to A+.

Question 87

What was the rationale for labeling bacteriophage with 35S and 32P in the Hershey and Chase ‘blender’ experiment?

Answer 87

35S labels protein, specifically since there is no S in nucleic acis. 32P labels nucleic acid specifically, since there is no P in the phage proteins.

Question 88

A plasmid that carries genes for its own transfer and propagations is called _____.

Answer 88

A plasmid that carries genes for its own transfer and propagation is called self-transmissible

Question 89

What enzymes can convert a supercoiled plasmid to a relaxed circle?

Answer 89

Helicases (topoisomerases) can digest the phosphodiester bond in one strand of the double-stranded DNA, allowing the twisted strands to unwind.

Question 90

Name three processing steps undergone by messenger RNA.

Answer 90

Three processing steps of mRNA are polyadenylation, capping, and splicing.

Question 91

What is the function of polyadenylate polymerase?

Answer 91

Polyadenylate polymerase digests RNA and adds adenines to the 3’ end of the transcript.

Question 92

What is unusual about the phosphodiester bond formed between mRNA and its 5’ cap?

Answer 92

The 5’ cap is attached by an unusual 5’ to 5’ pyrophosphate linkage.

Question 93

The parts of the hnRNA that are translated into protein (open reading frames) are the ______.

a. exons
b. introns
c. enhancers
d. miRNAs

Answer 93

a. exons

Question 94

The intervening sequences that interrupt protein coding sequences in the hnRNA are _____.

a. exons
b. introns
c. enhancers
d. miRNAs

Answer 94

b. introns

Question 95

Proteins that bind to DNA to control gene expression are called ______ .

a. restriction enzymes
b. cis factors
c. enhancers
d. trans factors

Answer 95

d. trans factors

Question 96

The binding sites on DNA for proteins that control gene expression are ______.

a. restriction enzymes
b. cis factors
c. enhancers
d. trans factors

Answer 96

b. cis factors

Question 97

How might a single mRNA produce more than one protein product?

Answer 97

A single RNA may be alternatively spliced to produce more than one product.

Question 98

The type of transcription producing RNA that is continually required and relatively abundant in the cell is called _____ transcription.

Answer 98

The type of transcription producing RNA that is continually required and relative abundant in the cell is called constitutive transcription.

Question 99

A set of structural genes transcribed together on one polycistronic mRNA is called _____.

Answer 99

A set of structural genes transcribed together on one polycistronic mRNA is called an operon.

Question 100

Would the methylation of cytosine bases 5’ to the gene increase or decrease expression of the gene?

Answer 100

Methylation of cytosine bases 5’ to the gene will decrease expression of the gene.

Question 101

Would histone acetylation close to the gene increase or decrease expression of the gene?

Answer 101

Histone acetylation close to the gene will increase expression

Question 102

What two factors are responsible for regulation of RNA synthesis?

Answer 102

cis factors, which are DNA sequences that mark places on DNA involved in the initiation and control of RNA synthesis
and
trans factors, which are proteins that bind to the cis sequences and direct the assembly of transcription complexes at the proper gene.

Question 103

Define Operon.

Answer 103

a series of structural genes transcribed together on one mRNA and subsequently separated into individual proteins. (e.g. in a small genome an operon might encode the enzymes of a metabolic pathway).

Question 104

What is encoded by the lac operon?

Answer 104

three structural genes, LacZ, LacY, and LacA, which are all required for the metabolism of lactose.
LacZ - beta-galactosidase (hydrolyzes lactose into glucose and galactose)
LacY - lactose permease (transports lactose into the cell)
LacA - thiogalactoside transacetylase (transacetylates galactosides)

Question 105

Name three modes of regulation for mRNA transcription in prokaryotes.

Answer 105

1. induction (e.g. lac operon)
2. repression (e.g. arg operon)
3. activation (e.g. mal operon)

Question 106

Name two distal regulatory elements for transcription.

Answer 106

enhancers and silencers

Question 107

Define star activity.

Answer 107

Under non-standard conditions, restriction enzymes can find and cut sequences that differ from their recognition sequences.

Question 108

Name five reaction conditions that an induce star activity.

Answer 108

1. suboptimal buffer
2. contamination with solvents or high concentrations of glycerol
3. prolonged reaction time
4. high concentration of enzymes
5. divalent cation imbalance

Question 109

Briefly explain Restriction Fragment Length Polymorphisms (RFLPs).

Answer 109

Given that inherited and somatic differences in human DNA, the number and location of restriction sites for a given restriction enzyme are not the same in all individuals. These differences in size or number of restriction fragments are called RFLPs.

Question 110

Name two uses for RFLPs (Restriction Fragment Length Polymorphisms).

Answer 110

Molecular-based human identification and analysis of structural changes in chromosomes (translocations, deletions, and insertions).

Question 111

Northern blots are used to determine:

a. gene structure
b. transcript structure
c. protein processing
d. DNA binding proteins

Answer 111

b. transcript structure
explanation: Northern blots target RNA using a nucleic acid probe and can determine transcript structure, processing, and gene expression.

Question 112

The Southern blot is used to determine:

a. gene structure
b. transcript structure
c. gene expression
d. protein processing

Answer 112

a. gene structure

Explanation: The Southern blot targets DNA using a nucleic acid probe to determine gene structure.

Question 113

Briefly explain the method of Southern blot.

Answer 113

DNA is isolated and cut with restriction enzymes. The fragments are separated by gel electrophoresis, denatured, and then transferred to a solid support (nitrocelluluose). DNA fragments are exposed to a labeled DNA or RNA probe that is complementary to the region of interest. The signal of the probe is detected and the presence of absence of the signal indicates whether the sequence in question is detected.

Question 114

A Southwestern blot:

a. Targets DNA with a nucleic acid probe
b. Targets RNA with a nucleic acid probe
c. Targets protein with a DNA probe
d. Targets protein with a protein probe

Answer 114

c. Targets protein with a DNA probe

A Southwestern blot targets Protein with a DNA probe to determine DNA binding proteins and gene regulation.

Question 115

A Western blot:

a. Targets DNA with a nucleic acid probe
b. Targets RNA with a nucleic acid probe
c. Targets protein with a DNA probe
d. Targets protein with a protein probe

Answer 115

D. Targets protein with a protein probe.
A Western is used to target protein with a protein probe (often an antibody) to determine protein processing and gene expression.

Question 116

A Northern blot:

a. Targets DNA with a nucleic acid probe
b. Targets RNA with a nucleic acid probe
c. Targets protein with a DNA probe
d. Targets protein with a protein probe

Answer 116

b. Targets RNA with a nucleic acid probe
A Northern blot targets RNA with a nucleic acid probe in order to determine transcript structure, processing, and gene expression.

Question 117

A Southern blot:

a. Targets DNA with a nucleic acid probe
b. Targets RNA with a nucleic acid probe
c. Targets protein with a DNA probe
d. Targets protein with a protein probe

Answer 117

a. targets DNA with a nucleic acid probe

A Southern blot targets DNA with a nucleic acid probe to determine gene structure.

Question 118

An Eastern blot:

a. Targets DNA with a nucleic acid probe
b. Targets RNA with a nucleic acid probe
c. Targets protein with a DNA probe
d. Targets protein with a protein probe

Answer 118

d. Targets protein with a protein probe
An Eastern blot targets protein with a protein probe as a modification of a Western blot. The assay uses an enzymatic detection (PathHunter (tm)); also, an Eastern blot can be used for the detection of specific agriculturally important proteins.

Question 119

What range of DNA input is commonly used for Southern blot analysis?

a. 5-10 ug
b. 10-20 ug
c. 10-50 ug
d. 30-100 ug

Answer 119

c. 10-50 ug
More or less DNA may be required depending on the sensitivity of the detection system, the volume and configuration of the wells, and the abundance of the target DNA. Also, in the clinical laboratory, specimen availability may limit the input DNA.

Question 120

Name three scenarios that might result in a complicated interpretation of a Southern blot.

Answer 120

a. degraded DNA (smear present)
b. incomplete cutting of restriction enzyme (anomalous patterns)
c. impurity in the DNA may result in a resistance to restriction digest

Question 121

In a Southern blot, if there is variation in the brightness of genomic DNA smears between lanes which is the best explanation?

a. not all DNA lanes were loaded with an equal amount of DNA
b. restriction enzyme activity was incomplete.
c. DNA is degraded.

Answer 121

a. not all DNA lanes were loaded with an equal amount of DNA.
The brightness of the DNA smears resulting from digestion with restriction enzymes digestion of genomic DNA should be similar from lane to lane, ensuring that equal amounts of starting DNA were added to each lane and reaction.

Question 122

In genomic DNA cut with restriction enzymes, what is the explanation if a large aggregate of DNA remains near the top of the lane when run on an agarose gel?

a. not all DNA lanes were loaded with an equal amount of DNA
b. restriction enzyme activity was incomplete.
c. DNA is degraded.

Answer 122

b. restriction enzyme activity was incomplete.

Question 123

In genomic DNA cut with restriction enzymes, what is the explanation if a smear is located primarily in the lower region of the lane on an agarose gel?

a. not all DNA lanes were loaded with an equal amount of DNA
b. restriction enzyme activity was incomplete.
c. DNA is degraded.

Answer 123

c. DNA is degraded.

Question 124

What is the difference between the two results obtained from a Southern blot: the smeared appearance and the banded fragments?

Answer 124

The smeared agarose gel is viewed with UV to determine if the restriction digestion was successful. The banded or resolved appearance follows transfer of the agarose gel to a membrane that is then probed with a known single-stranded DNA or RNA labeled probe.

Question 125

Describe briefly the process of depurination of a Southern blot and why it is important.

Answer 125

before moving DNA fragments to a membane, the double-stranded DNA must be denatured into single-stranded DNA to bind to the probe. Short fragments (>500 bp) are denatured by exposing the gel to a strong base (sodium hydroxide), which promotes the breakage of the hydrogen bonds holding the DNA strands together. Large fragments are more efficiently denatured if they are depurinated first. Depurination requires soaking the gel in hydrogen chloride (HCL), which removed purine bases from the sugar-phosphate backbone. This loosens the larger fragments for denaturation with a strong base (sodium hydroxide).

Question 126

Why is nitrocellulose the membrane of choice for Southern blots?

Answer 126

ss-DNA binds to nitrocellulose membranes with a noncovalent, but irreversible, connection. The binding interaction is hydrophobic and electrostatic between the negatively charged DNA and the positive charge on the membrane.

Question 127

Why is it possible to reprobe a Southern blot?

Answer 127

Because the bond between the membrane and the DNA is much stronger than the hydrogen bonds that hold the complementary probe to the DNA.

Question 128

Briefly describe capillary transfer for Southern blots.

Answer 128

Capillary transfer is a simple and relatively inexpensive. The buffer moves from the bottom of the reservoir by capillary action through the gel, through the membrane and then through dry paper on top of the membrane. When the DNA comes in contact with the membrane it will bind to it. Issues with this method are bubbles, crystals, or other particulates that might be between the membrane and the gel will cause staining artifacts or loss of information. Also, this procedure is slow and usually takes overnight.

Question 129

What is the purpose of the prehybridization step in Southern blot analysis?

Answer 129

The purpose of the prehybridization step is to prevent the probe from binding to nonspecific sites on the membrane surface, which will cause high background noise.

Question 130

Name at two blocking agents for a Southern blot.

Answer 130

Denhardt solution (Ficoll, polyvinyl pyrrolidane, bovine serum albumin) and salmon sperm DNA.

Question 131

What is the best gel type to resolve small nucleic acid fragments?

a. Acrylamide
b. Agarose
c. Poly-acrylamide

Answer 131

c. poly-acrylamide
Poly-acrylamide is a combination of acrylamide and the cross-linker methylene bisacrylamide that gives consistent resolution characteristics.