Deck 7: Recombinant Dna and Biotechnology

A) detection of exon deletions.
B) amplification of a target DNA sequence.
C) in vivo correction of a mutated gene.
D) detection of trinucleotide repeat expansions.

A) contains DNA sequences from all species.
B) contains plasmid DNA copies of human total RNA.
C) contains amplified copies of a specific gene.
D) is often constructed using phage lambda.
E) is often screened by Southern blot hybridization.

A) origin of replication.
B) selectable marker.
C) bacterial promoter.
D) polyadenylation signal.
E) Shine_Dalgarno sequence.

A) The gene is at least one cM from the RFLP.
B) The gene is homozygous in the affected individual.
C) The gene contains a nonsense mutation.
D) The gene is heterozygous in the individual.
E) The gene contains numerous polymorphisms.

A) Taq polymerase can synthesize only 1000 base pairs of DNA at a time.
B) polymerization proceeds to the ends of the DNA.
C) Taq polymerase is denatured after each cycle is complete.
D) the DNA is cut with restriction enzymes prior to PCR.
E) the reaction contains a limiting amount of nucleoside triphosphate precursors.

A) DNA ligase.
B) bacteriophage lambda.
C) reverse transcriptase.
D) restriction enzymes.

A) terminal transferase.
B) ligase.
C) RNA-dependent DNA polymerase.
D) DNA-dependent RNA polymerase.
E) kinase.

A) Southern blot analysis.
B) colony hybridization.
C) restriction enzyme digestion.
D) agarose gel electrophoresis.
E) ethidium bromide treatment.

A) centromeric sequences.
B) telomeric sequences.
C) an origin of replication.
D) a locus control region.
E) a selectable marker gene.

A) they cleave double stranded DNA.
B) they modify DNA by methylation.
C) they recognize specific DNA sequences.
D) they cleave DNA, producing staggered ends.

A) requires that cDNA inserts have been used in the library being screened.
B) requires the utilization of vector sequences that provide high efficiency translation of the cloned insert DNA including signals for initiation and termination of translation.
C) requires the utilization of vector sequences that provide high efficiency transcription of the cloned insert DNA including signals for initiation and termination of transcription.
D) will isolate any gene that encodes a protein product recognized by the antibody.
E) all of the above statements are true.

A) gel shift assay.
B) dideoxy chain termination.
C) Southern blotting.
D) DNA ligation.
E) Northern blotting.

A) allows specific chemical cleavage of the DNA strand at random sites.
B) is required for the synthesis of the primer.
C) causes termination of DNA chain elongation.
D) cannot be utilized by DNA polymerase.
E) lacks a 5' phosphate group.

A) identification of point mutations.
B) detection of deleted exons.
C) linkage analysis.
D) detection of trinucleotide repeat expansions.

A) they recognize specific palindromic sequences.
B) they may produce staggered ends when they cleave DNA into fragments.
C) they may produce flush ends when they cleave DNA into fragments.
D) they are used in gene cloning to cleave the single stranded regions of the cDNA produced by reverse transcriptase.
E) they are used to cleave plasmid DNA in specific places in gene cloning experiments.

A) DNA polymerases
B) RNA polymerases
C) endonucleases
D) exonucleases
E) none of the above

A) Double strand breakage and rejoining of nonhomologous chromosomes
B) Double_strand breakage and rejoining of homologous chromosomes
C) Single-strand breakage and strand transfer between non-homologous chromosomes
D) Single_strand breakage and strand transfer between homologous chromosomes

A) gel shift assay.
B) dideoxy chain termination.
C) Southern blotting.
D) DNA ligation.
E) Northern blotting.

A) remove single stranded DNA and repair the restriction enzyme site after transformation respectively.
B) make cDNA and create sticky ends on the cDNA and the staggered ends of the cleaved restriction site.
C) repair the restriction enzyme site before transformation.
D) repair the restriction enzyme site after transformation.
E) remove the sticky ends prior to the DNA ligase step.

A) recombination can only occur at Chi sites
B) recombination only occurs at specific DNA sequences
C) recombination requires a single_stranded region and a duplex DNA region with closely related DNA sequence
D) recombination requires an RNA intermediate
E) recombination is site-specific

A) The TATA box-binding protein, TBP, which binds within the minor groove.
B) Retrovirus proviral DNA, which integrates within the major groove.
C) Topoisomerase II, which binds to the sugar-phosphate backbone.
D) SV40 large T-antigen, which binds to the major groove.
E) None of the above.

A) Southern blot analysis.
B) Colony hybridization
C) Restriction enzyme digestion.
D) Agarose gel electrophoresis.
E) Ethidium bromide treatment

A) rescue of mutants.
B) generation of chemically_induced mutant loci.
C) synthetic bioreactors.
D) testing drug or gene therapies.
E) studies of structure_function relationships.

A) DNA polymerase + DNA ligase
B) DNA polymerase + RNA polymerase
C) Restriction enzyme + DNA ligase
D) Phosphorylase + DNA ligase
E) Acetylase + single stranded DNA specific deoxyribonuclease

A) RFLP linkage analysis
B) Allele specific oligonucleotide (ASO) analysis
C) Fluorescence in situ hybridization (FISH)
D) Multiplex PCR

A) introns.
B) exons.
C) promoters.
D) spliced sequences.
E) Alu sequences.

A) bacteriophage and HIV
B) DNA viruses and RNA viruses
C) adenoviruses and foamy viruses
D) influenza viruses and liposomes

A) unwinds double stranded DNA by breaking base pairs
B) will decrease the writhing number of negatively supercoiled DNA
C) will decrease the linking number of negatively supercoiled DNA
D) nicks one strand of double stranded DNA
E) cuts both strands of double stranded DNA

A) Labeling reactions are initiated by synthetic oligonucleotides.
B) The incorporation of labeled precursor involves an in vitro DNA replication reaction.
C) Nuclease activity can degrade newly synthesized, labeled DNA.
D) They both incorporate -labeled ribonucleotides.

A) dNTPs
B) dideoxynucleotides
C) AZT
D) DNA polymerase

A) play a role in the repair of DNA.
B) generate new combinations of genes.
C) generate point mutations.
D) regulate the expression of DNA.
E) involve single strand breaks.

A) It will identify which RNA in a population is complementary to a specific DNA probe.
B) It is used to purify a gene by electrophoretic separation from a population of genes.
C) It is useful for repetitive DNA but not unique sequence DNA.
D) It is used to amplify a specific DNA sequence in vitro.
E) It identifies a specific fragment of DNA based on complementarity to a radioactive DNA probe.

A) preparation of large amounts of DNA for structural analysis.
B) preparation of proteins such as alpha globin, insulin, and interferon.
C) creation of phage collections which, in total, represent the entire genome of an organism.
D) prenatal identification of some genetic diseases.
E) repair of genetic damage caused by radiation.

A) ensures that the DNA fragments being cloned are very small.
B) ensures that introns are separated from exons.
C) generates overlapping fragments of the genome.
D) separates repetitive sequences from unique sequences.

A) Genomic library
B) DNA sequence analysis
C) Comparison of the normal and mutant genes
D) Prior knowledge of the protein product
E) Overlapping genomic clones

A) The fibroin gene undergoes DNA amplification within moth silk gland cells to enable the synthesis of up to 109 silk fibroin proteins per cell.
B) Up to 98% of the human genome encodes proteins and structural RNA's.
C) Histone genes are tandemly repeated and localized in nucleoli.
D) Amplification of protein- encoding genes is commonly seen during amphibian oogenesis, when enormous stores of protein are needed.
E) Eukaryotic chromosomes each consist of a single linear DNA molecule.

A) a cDNA library in pBR.
B) a cDNA library in an expression vector.
C) a genomic DNA library cloned into a YAC vector.
D) a cDNA library cloned into a YAC vector.
E) a genomic DNA library cloned into a phage vector.

A) promoter
B) ribosome binding site
C) initiation codon
D) DNA-dependent RNA polymerase II
E) coli?

A) synthesis of ribosomal RNA from pre-existing ribosomal RNA
B) synthesis of RNA primers for Okazaki fragments
C) synthesis of RNA using a single stranded RNA template
D) synthesis of mRNA from double stranded viral RNA
E) synthesis of DNA using a RNA template

A) chemical base-modification reactions to fragment the DNA.
B) base-specific enzymes to obtain the sequence.
C) families of restriction enzymes of known specificity to obtain the sequence.
D) alkaline hydrolysis and thin layer chromatography to obtain the base composition.
E) reassociation kinetics to determine the sequence complexity of DNA.

A) contain negatively supercoiled DNA.
B) consist of linear DNA polynucleotide chains.
C) contain both repetitive and nonrepetitive DNA.
D) contain nucleosomes spaced approximately 200 bp apart.
E) contain restriction enzymes.

A) each of the arms of the Chi structure will be a different length
B) each of the arms will be the same length
C) two of the arms will be the same length and the other two arms will be the same length
D) three of the arms will be the same length and the fourth arm will be a different length
E) none of the above are true

A) exchange of genetic information between nonhomologous chromosomes.
B) reciprocal translocation of unlike DNA between sister chromatids.
C) conversion of one allele to another by DNA repair.
D) exchange of genetic information between homologous chromosomes.

A) copies of genes.
B) mRNAs.
C) fragments of genomic DNA.
D) DNA copies of mRNA.
E) intron DNA sequences.

A) knock-in mutation.
B) transgenesis.
C) nuclear transfer.
D) transposition.
E) knockout mutation.

A) classical genetic mapping.
B) DNA fingerprinting.
C) locating a disease gene.
D) prenatal screening for a possible genetic defect.
E) creating a cDNA library.

A) one of two recombination products are formed depending on how the branch is cleaved
B) strand exchange leads to an intermediate structure with crossed single strands
C) two homologous duplexes are aligned
D) the branch can move along the strands leading to additional strand exchange
E) the strand exchange is initiated by DNase I nicking.

A) the activity of DNA polymerase
B) the use of chemical agents that modify DNA
C) the transfer of electrophoretically resolved DNA to a nitrocellulose filter.
D) the incorporation of poly dT the 3'-OH end of a DNA strand.

A) composed of a mixture of different oligonucleotide sequences.
B) composed only of the most frequently used codon for each amino acid.
C) completely random oligonucleotide sequences.
D) small restriction enzyme fragments.

A) viruses.
B) non-tumor forming RNA viruses.
C) single stranded RNA viruses.
D) segmented-genome viruses.

A) digestion of total human DNA with restriction endonucleases, separation of fragments by gel electrophoresis and hybridization with a labeled gene probe.
B) somatic cell hybridization.
C) isolation of fetal messenger RNA and in vitro translation.
D) None of the above techniques could yield such information.

A) Those that have been treated with a drug regimen.
B) Those that are bred for polymorphic alleles of one gene.
C) Clones derived by nuclear transfer.
D) Those that carry a foreign gene that was deliberately inserted into their genomes.
E) Those that are infected with a virus to test vaccine efficacy.

A) DNA sequence specifically.
B) each DNA strand separately.
C) palindromic sequences.
D) DNA using an exonuclease activity.

A) challenges to successful gene therapy.
B) techniques used to study developmental regulation.
C) protocols used in the production of transgenic and chimeric mice.
D) problems encountered in the development of pharmaceuticals.

A) origin of replication
B) selectable marker
C) bacterial promoter
D) polyadenylation signal
E) Shine-Dalgarno sequence

A) restriction endonucleases and DNA ligase.
B) restriction endonucleases and Pol I.
C) Pol I and DNA ligase.
D) recombinase and DNA gyrase.

A) direct physical interaction between the ribosome and RNA polymerase.
B) pausing of a ribosome in the leader peptide due to low levels of an operon-specific charged tRNA.
C) no proteins other than those in ribosomes and RNA polymerase.
D) the formation of a stem loop structure in the nascent mRNA strand that acts as a transcriptional terminator.

A) Vectors such as plasmids or bacterial viruses can be used for cloning foreign DNA in bacterial cells.
B) Recombinant molecules between plasmid DNA and foreign DNA can be generated by using restriction endonucleases.
C) cDNA synthesized from the messenger RNA of a desired gene can be cloned.
D) If foreign DNA is inserted into a bacterial plasmid, the recombinant plasmid cannot be used for transforming eukaryotic cells.
E) Some eukaryotic genes can be expressed when transformed into bacteria.

A) a cDNA construct encoding LDL, under the control of a bacterial promoter
B) the human gene encoding LDL, under the control of a bacterial promoter
C) a cDNA construct encoding LDL, under the control of the LDL promoter
D) the human gene encoding LDL, under the control of the LDL promoter

A) The entire protein coding sequence of the gene.
B) A sequence complementary to the 3' poly-A tail of the mRNA encoded by the gene.
C) The chromosome containing the gene.
D) A segment of intron DNA.

A) Each primer needs to base-pair with a site on one of the two DNA strands.
B) The primers need to base-pair with each other.
C) Each primer needs to base-pair with two sites on each of the two DNA strands.
D) The two primers need to base-pair with sites that are repetitive in the genome.

A) bacteria possess the necessary enzymes to correctly process the primary transcript containing intron sequences.
B) a cDNA copy of the mRNA can be cloned and expressed.
C) the protein synthetic machinery of the bacteria will only translate the exon portions of the resulting RNA.
D) the translation of intron regions will not alter the activity of the protein if they are removed by proteolytic processing.

A) is a viral DNA polymerase.
B) requires a primer.
C) uses either DNA or RNA as a template.
D) synthesizes both DNA and RNA.

A) the synthesis of nucleotides from bases and sugar-phosphates.
B) the hydrolysis of nucleotides to nucleosides and inorganic phosphate.
C) the hydrolysis of cyclic AMP.
D) the synthesis of a polynucleotide chain from nucleotide units.
E) the hydrolysis of internucleotide linkages of a polynucleotide chain.

A) length.
B) sequence.
C) GC content.
D) AT content.
E) density.

A) They contain null mutations in mouse genes.
B) They are generated by homologous recombination of a gene targeting vector in embryonic stem cells.
C) The initial mice produced are chimeric.
D) The effects of the mutations are usually pleiotropic.
E) The mutations are usually lethal during the embryonic stage of development.

A) compare polypeptide conformation.
B) prepare large, unilamellar lipid vesicles.
C) determine enzyme turnover numbers.
D) establish DNA sequence homologies.
E) investigate ribosome assembly.

A) are compatible with YAC vectors.
B) contain non-contiguous but linearly related fragments.
C) can be amplified by the polymerase chain reaction.
D) contain unclonable sequences.

A) Taq polymerase can only synthesize DNA of discrete size from any DNA template.
B) the reaction is terminated by denaturation at the same time following each round of polymerization.
C) the primers are of discrete size.
D) of the exponential production of run-off products.
E) the template for amplification is always a specific cloned DNA fragment.

A) Mice are physiologically similar to humans.
B) New diseases can be induced in mice for which there is no human counterpart yet.
C) They allow the study of polygenic disease.
D) Technology advances have increased the ability to create mouse models of human disease.
E) A large reservoir of potential models exists in spontaneous or induced mutant loci.

A) ApTpGpCpCpGpTpAp
B) GpCpTpApTpGpApCp
C) ApTpGpCpTpApCpGp
D) GpTpCpApTpGpApCp

A) isolation of human beta globin mRNA.
B) use of poly dT as a primer for reverse transcriptase.
C) transcription with
D) homopolymer tailing of the cDNA and ligation of the tailed cDNA to the vector.
E) coli RNA polymerase.

A) No radioactivity would be detected in either cells or supernatant.
B) The radioactivity would be found in the progeny phage particles if infection of the cells was allowed to continue.
C) The supernatant fluid would contain most of the radioactivity
D) The radioactivity would be found in the phage DNA within the infected cells

A) genomic DNA from specific tissues.
B) reverse transcribed cellular RNA.
C) reverse translated cellular proteins.
D) reverse transcriptase.
E) satellite DNA.

A) very small size
B) multiple copies are incorporated per cell
C) codes for the protein required for tetracycline resistance
D) contains three sites for the restriction endonuclease to be used

A) ensures that the DNA fragments being cloned are very small.
B) ensures that introns are separated from exons.
C) generates overlapping fragments of the genome.
D) separates repetitive sequences from unique sequences.

A) digest DNA duplex molecules from the 5'-OH ends.
B) attack only single stranded DNA.
C) have base sequence specificity.
D) randomly digest double stranded DNA molecules.
E) are not produced by bacteria.

A) RNA directed DNA synthesis.
B) DNA directed DNA synthesis.
C) DNA directed RNA synthesis.
D) Hydrolysis of RNA.

A) to determine restriction fragment sizes.
B) to detect deleted genes.
C) to detect gene rearrangements.
D) to measure mRNA size.