Deck 21: Genetics of Complex Traits

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Question
Which of the following is an important control component when using an RNAi library to screening breast cancer cell lines for genes required for cell profileration?

A) genomic DNA
B) Cy3 dyes
C) Cy5 dyes
D) a normal mammary cell line
E) barcodes
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Question
Genes that are synthetic lethal most likely function in

A) rapidly evolving pathways
B) dispensable processes
C) the same pathway
D) reproductive pathways
E) parallel pathways
Question
Approximately what proportion of genes have been shown to be essential for viability in yeast?

A) 20%
B) 40%
C) 50%
D) 60%
E) 80%
Question
Barcodes are used in knock-out and knock-down screen in both yeast cells and human cells.
Question
Which of the following is a property of Saccharomyces cerevisiae but not Caenorhabditis elegans?

A) sexual reproduction
B) multicellularity
C) fully sequenced genome
D) efficient homologous recombination
E) ability to take up foreign DNA
Question
If A- is the genotype of a query strain,the genotype that is tested for synthetic lethality in a synthetic genetic array is:

A) A-A-
B) A-B+
C) A-B-
D) A+A-
E) A-A-B- B-
Question
Approximately how many digenic mutant combinations result in a lethal phenotype in budding yeast?

A) 1,000
B) 2,500
C) 25,000
D) 100,000
E) 250,000
Question
What is the difference between siRNA and shRNA?

A) siRNA is used for eukaryotes;shRNA is used for prokaryotes
B) siRNA is used for stable silencing;shRNA is used for transient silencing
C) siRNA is 50 nucleotides;shRNA 19-22 bp
D) siRNA is ssRNA;shRNA is dsRNA
E) siRNA is chemically synthesized;shRNA is delivered to the cell as a plasmid
Question
A diagram showing all of the functional overlap between genes of a given species can be used to describe its

A) synthetic array.
B) genome architecture.
C) genotype-phenotype relationships.
D) phenological array.
E) phylogenetic history.
Question
In a synthetic lethal,which of the following phenotypes is most likely to be non-viable?

A) A+B+
B) A-B+
C) A+B-
D) A-B-
E) A+A-B+ B+
Question
Why is Saccharomyces cerevisiae a useful model organism for functional genetics?

A) It has approximately the same number of protein coding genes as humans do.
B) It has the smallest genome of any organism.
C) The function of every one of its genes is known.
D) It has the smallest genome of any eukaryote.
E) It can exist as a haploid or diploid.
Question
Where should barcodes be placed in a gene deletion cassette?

A) flanking the selectable marker
B) flanking one of the homologous fragments
C) flanking both homologous fragments
D) in the middle of the selectable marker
E) in the middle of the homologous fragment
Question
shRNA is a type of RNAi.
Question
Which of the following is the correct order of steps in a synthetic genetic array screen?

A) mating,sporulation,kanR selection,assay double mutants
B) sporulation,kanR selection,mating,assay double mutants
C) mating,kanR selection,assay double mutants,sporulation
D) kanR selection,assay double mutants,mating,sporulation
E) mating,kanR selection,sporulation,assay double mutants
Question
Genetic buffering describes

A) the ability of cells to accumulate mutations.
B) loss of mutations through repair and recombination.
C) the accumulation of extra,non-coding DNA in eukaryotic genomes.
D) the ability of one gene to mask variability in another gene.
E) the expansion of introns throughout evolution.
Question
Which of the following statements about shRNA is not true?

A) shRNAs are synthetic 19-22bp dsRNAs.
B) shRNA encodes a substrate of RISC.
C) shRNAs encodes ssRNA.
D) shRNA is used to produce siRNA.
E) shRNA can be packaged into a virus.
Question
You grow a barcoded yeast deletion set at 4°C and then a copy of the same set at 25°C.Barcodes from the 4°C sample and 25°C are labeled with a green fluorochrome and a red fluorochrome,respectively.How will you identify genes required for growth specifically at cold temperatures?

A) separate the PCR products on an agarose gel and look for red fluorescent bands
B) separate the PCR products on an agarose gel and look for yellow fluorescent bands
C) hybridize the products to a microarray and look for red spots
D) hybridize the products to a microarray and look for green spots
E) separate the PCR products on an agarose gel and look for green fluorescent bands
Question
Synthetic genetic arrays involve mating a ________ with __________.

A) haploid wild-type;all inviable deletion mutants.
B) diploid query strain;a haploid wild-type strain.
C) haploid query strain;a diploid wild-type.
D) haploid query strain;all viable haploid deletion mutants.
E) inviable diploid strain;all viable haploid deletion mutants.
Question
Which of these would be of the least use in a gene deletion cassette for use in yeast?

A) kanR gene
B) DNA barcode
C) common PCR primer binding sites
D) shRNA
E) yeast DNA sequences
Question
Which of the following is not true of the most highly connected nodes in a genetic interaction map?

A) they are the minority of nodes
B) they are also known as hubs
C) they have a greater influence on phenotype than other genes
D) they typically show scale-free architecture
E) they have lowest buffering capacity of any genes
Question
Explain why budding yeast (Saccharomyces cerevisiae)is a particularly useful tool for functional genomics.What are the limitations of budding yeast as model organism?
Question
Genes of round worms (Caenorhabitis elegans)can be silenced by soaking the worms in siRNA.
Question
siRNA contains a stem loop.
Question
Budding yeast with the genotype A+B+ is haploid.
Question
A comprehensive collection of deletion mutants is required for synthetic genetic array analysis.
Question
How are the gene interaction maps that are made by analysis of synthetic genetic arrays related to protein interaction maps made by e.g.yeast two-hybrid analysis?
Question
Retroviruses can be used for targeted gene silencing in mammal cells.
Question
In scale-free networks,the number of links shows a normal distribution.
Question
In genetic interaction maps,most genes have the same number of links to other genes.
Question
The analysis of genetic architecture in model organisms indicates that complex phenotypes are controlled by relatively few genes.
Question
RNAi techniques completely knock-out the transcription of their target gene.
Question
How could you use shRNA and human cell lines to identify genes to target for cancer therapy? Discuss the methods and expected results and your intepretations.
Question
Compare genome sequencing,functional genomics,and systems biology.
Question
There are more mutant combinations that cause lethality than there are single mutants that cause lethality.
Question
Modifiers in genetic networks control the strength of mutant phenotypes.
Question
Up to 85% of introduced deletion casettes will undergo homologous recombination in budding yeast.
Question
One pair of PCR primers can amplify any of the barcodes in the genome-wide yeast deletion set.
Question
In a genetic interaction map,a line connects two genes that are both required for normal growth.
Question
Two crossovers are usually involved when using a yeast deletion cassette to knock-out a gene.
Question
Because it cannot be automated,image analysis is the major limitation in phenotyping genome-wide yeast deletion analysis.
Question
How would the methods for genome-wide deletion screens change if barcodes were not available?
Question
What do synthetic genetic arrays reveal about the function of genes in general?
Question
What is the benefit of using barcodes in genome-wide deletion screens?
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Deck 21: Genetics of Complex Traits
1
Which of the following is an important control component when using an RNAi library to screening breast cancer cell lines for genes required for cell profileration?

A) genomic DNA
B) Cy3 dyes
C) Cy5 dyes
D) a normal mammary cell line
E) barcodes
D
2
Genes that are synthetic lethal most likely function in

A) rapidly evolving pathways
B) dispensable processes
C) the same pathway
D) reproductive pathways
E) parallel pathways
E
3
Approximately what proportion of genes have been shown to be essential for viability in yeast?

A) 20%
B) 40%
C) 50%
D) 60%
E) 80%
A
4
Barcodes are used in knock-out and knock-down screen in both yeast cells and human cells.
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5
Which of the following is a property of Saccharomyces cerevisiae but not Caenorhabditis elegans?

A) sexual reproduction
B) multicellularity
C) fully sequenced genome
D) efficient homologous recombination
E) ability to take up foreign DNA
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
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6
If A- is the genotype of a query strain,the genotype that is tested for synthetic lethality in a synthetic genetic array is:

A) A-A-
B) A-B+
C) A-B-
D) A+A-
E) A-A-B- B-
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7
Approximately how many digenic mutant combinations result in a lethal phenotype in budding yeast?

A) 1,000
B) 2,500
C) 25,000
D) 100,000
E) 250,000
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
8
What is the difference between siRNA and shRNA?

A) siRNA is used for eukaryotes;shRNA is used for prokaryotes
B) siRNA is used for stable silencing;shRNA is used for transient silencing
C) siRNA is 50 nucleotides;shRNA 19-22 bp
D) siRNA is ssRNA;shRNA is dsRNA
E) siRNA is chemically synthesized;shRNA is delivered to the cell as a plasmid
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
9
A diagram showing all of the functional overlap between genes of a given species can be used to describe its

A) synthetic array.
B) genome architecture.
C) genotype-phenotype relationships.
D) phenological array.
E) phylogenetic history.
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
10
In a synthetic lethal,which of the following phenotypes is most likely to be non-viable?

A) A+B+
B) A-B+
C) A+B-
D) A-B-
E) A+A-B+ B+
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
11
Why is Saccharomyces cerevisiae a useful model organism for functional genetics?

A) It has approximately the same number of protein coding genes as humans do.
B) It has the smallest genome of any organism.
C) The function of every one of its genes is known.
D) It has the smallest genome of any eukaryote.
E) It can exist as a haploid or diploid.
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
12
Where should barcodes be placed in a gene deletion cassette?

A) flanking the selectable marker
B) flanking one of the homologous fragments
C) flanking both homologous fragments
D) in the middle of the selectable marker
E) in the middle of the homologous fragment
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
13
shRNA is a type of RNAi.
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Unlock Deck
k this deck
14
Which of the following is the correct order of steps in a synthetic genetic array screen?

A) mating,sporulation,kanR selection,assay double mutants
B) sporulation,kanR selection,mating,assay double mutants
C) mating,kanR selection,assay double mutants,sporulation
D) kanR selection,assay double mutants,mating,sporulation
E) mating,kanR selection,sporulation,assay double mutants
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
15
Genetic buffering describes

A) the ability of cells to accumulate mutations.
B) loss of mutations through repair and recombination.
C) the accumulation of extra,non-coding DNA in eukaryotic genomes.
D) the ability of one gene to mask variability in another gene.
E) the expansion of introns throughout evolution.
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
16
Which of the following statements about shRNA is not true?

A) shRNAs are synthetic 19-22bp dsRNAs.
B) shRNA encodes a substrate of RISC.
C) shRNAs encodes ssRNA.
D) shRNA is used to produce siRNA.
E) shRNA can be packaged into a virus.
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
17
You grow a barcoded yeast deletion set at 4°C and then a copy of the same set at 25°C.Barcodes from the 4°C sample and 25°C are labeled with a green fluorochrome and a red fluorochrome,respectively.How will you identify genes required for growth specifically at cold temperatures?

A) separate the PCR products on an agarose gel and look for red fluorescent bands
B) separate the PCR products on an agarose gel and look for yellow fluorescent bands
C) hybridize the products to a microarray and look for red spots
D) hybridize the products to a microarray and look for green spots
E) separate the PCR products on an agarose gel and look for green fluorescent bands
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
18
Synthetic genetic arrays involve mating a ________ with __________.

A) haploid wild-type;all inviable deletion mutants.
B) diploid query strain;a haploid wild-type strain.
C) haploid query strain;a diploid wild-type.
D) haploid query strain;all viable haploid deletion mutants.
E) inviable diploid strain;all viable haploid deletion mutants.
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
19
Which of these would be of the least use in a gene deletion cassette for use in yeast?

A) kanR gene
B) DNA barcode
C) common PCR primer binding sites
D) shRNA
E) yeast DNA sequences
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
20
Which of the following is not true of the most highly connected nodes in a genetic interaction map?

A) they are the minority of nodes
B) they are also known as hubs
C) they have a greater influence on phenotype than other genes
D) they typically show scale-free architecture
E) they have lowest buffering capacity of any genes
Unlock Deck
Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
21
Explain why budding yeast (Saccharomyces cerevisiae)is a particularly useful tool for functional genomics.What are the limitations of budding yeast as model organism?
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
22
Genes of round worms (Caenorhabitis elegans)can be silenced by soaking the worms in siRNA.
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k this deck
23
siRNA contains a stem loop.
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k this deck
24
Budding yeast with the genotype A+B+ is haploid.
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k this deck
25
A comprehensive collection of deletion mutants is required for synthetic genetic array analysis.
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k this deck
26
How are the gene interaction maps that are made by analysis of synthetic genetic arrays related to protein interaction maps made by e.g.yeast two-hybrid analysis?
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
27
Retroviruses can be used for targeted gene silencing in mammal cells.
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Unlock Deck
k this deck
28
In scale-free networks,the number of links shows a normal distribution.
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k this deck
29
In genetic interaction maps,most genes have the same number of links to other genes.
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k this deck
30
The analysis of genetic architecture in model organisms indicates that complex phenotypes are controlled by relatively few genes.
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Unlock Deck
k this deck
31
RNAi techniques completely knock-out the transcription of their target gene.
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k this deck
32
How could you use shRNA and human cell lines to identify genes to target for cancer therapy? Discuss the methods and expected results and your intepretations.
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
33
Compare genome sequencing,functional genomics,and systems biology.
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Unlock for access to all 43 flashcards in this deck.
Unlock Deck
k this deck
34
There are more mutant combinations that cause lethality than there are single mutants that cause lethality.
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k this deck
35
Modifiers in genetic networks control the strength of mutant phenotypes.
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k this deck
36
Up to 85% of introduced deletion casettes will undergo homologous recombination in budding yeast.
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k this deck
37
One pair of PCR primers can amplify any of the barcodes in the genome-wide yeast deletion set.
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k this deck
38
In a genetic interaction map,a line connects two genes that are both required for normal growth.
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k this deck
39
Two crossovers are usually involved when using a yeast deletion cassette to knock-out a gene.
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k this deck
40
Because it cannot be automated,image analysis is the major limitation in phenotyping genome-wide yeast deletion analysis.
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k this deck
41
How would the methods for genome-wide deletion screens change if barcodes were not available?
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42
What do synthetic genetic arrays reveal about the function of genes in general?
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43
What is the benefit of using barcodes in genome-wide deletion screens?
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