Deck 9: Biotechnology and Recombinant DNA

A)exonucleases.
B)proteases.
C)restriction enzymes.
D)RNA polymerases.

A)nigrosin.
B)malachite green.
C)gold oxide.
D)ethidium bromide.

A)is always donated to the offspring from both parents.
B)can be used to identify related people.
C)can be isolated only from intact embryos.
D)can be used to establish paternity.

A)S.aureus.
B)rhinovirus.
C)coli.

A)book of genes.
B)recombinant gene.
C)DNA library.
D)restructured genome.

A)interacts electrically with the DNA.
B)chemically binds to the DNA.
C)acts as a sieve.
D)selectively sorts recombinant DNA from host DNA.

A)biotechnology.
B)gene cloning.
C)recombinant DNA.
D)genetic engineering.

A)density.
B)shape.
C)size.
D)sequence.

A)may be a plasmid or bacteriophage.
B)has a restriction enzyme recognition site.
C)contains an origin of replication.
D)contains a selectable marker.
E)All of the choices are correct.

A)DNAse.
B)DNA ligase.
C)ligandase.
D)polymerase.
E)DNAse AND ligandase.

A)allows the use of bacteria as production factories for a number of molecules.
B)relies on recombinant DNA technology.
C)is dependent on RNA enzymes.
D)relies completely on conjugation.
E)allows the use of bacteria as production factories for a number of molecules AND relies on recombinant DNA technology.

A)they cut at defined sites.
B)the sticky ends make it very easy to allow recombination of any type of DNA.
C)they protect eukaryotes against virus attack.
D)they cut RNA molecules.
E)they cut at defined sites AND the sticky ends make it very easy to allow recombination of any type of DNA.

A)gravity.
B)active transport.
C)agarosis.
D)electricity.

A)pest-resistant plants.
B)plants that are herbicide resistant.
C)plants with increased nutritional value.
D)All of the choices are correct.

A)identifying organisms that have taken up recombinant DNA.
B)searching for RNA.
C)production of proteins.
D)production of DNA.

A)produces sticky ends.
B)produces blunt ends.
C)cuts both strands of the DNA molecule.
D)generates restriction fragments.
E)All of the choices are correct.

A)bacteria.
B)viruses.
C)nucleotides.
D)plasmids.
E)viruses AND plasmids.

A)are useful in identifying specific individuals.
B)are important sites in vectors where foreign DNA can be integrated.
C)are errors that can arise during DNA sequencing.
D)are DNA fragments generated during PCR.

A)red colonies.
B)white colonies.
C)blue colonies.
D)All of the choices are correct.

A)DNA fragments of all possible sizes.
B)DNA fragments that are one nucleotide larger than the next fragment.
C)DNA fragments of a particular size.
D)DNA fragments of increasing size.
E)DNA fragments that are one nucleotide larger than the next fragment AND DNA fragments of increasing size.

A)about $10
B)about $1,000
C)about $1,000,000
D)over $400,000,000

A)detecting viable yet non-culturable organisms.
B)assessing impure (multiple types of bacteria present)samples.
C)dealing with very small numbers of bacteria.
D)relatively quickly producing results.
E)All of the choices are correct.

A)it contains radioactive particles.
B)it may contain some unanticipated allergens.
C)it may have some unintended environmental effects.
D)the modified DNA may transfer to other organisms.
E)it may contain some unanticipated allergens,it may have some unintended environmental effects,AND the modified DNA may transfer to other organisms.

A)how many cycles are performed.
B)the size of the template DNA.
C)the location to which the primers anneal.
D)how much Taq is used.

A)2 additional pieces of dsDNA.
B)4 additional pieces of dsDNA.
C)8 additional pieces of dsDNA.
D)16 additional pieces of dsDNA.

A)a protein.
B)many copies of the gene to be used as a probe.
C)many copies of the gene for sequencing.
D)more copies of the host cell.
E)a protein,many copies of the gene to be used as a probe,AND many copies of the gene for sequencing.

A)DNA.
B)RNA.
C)proteins.
D)lipids.

A)vector.
B)probe.
C)host.
D)plasmid.
E)coli that carries the desired recombinant DNA is by using a

A)may use many DNA fragments that function like probes.
B)attaches nucleotides to a solid support such as a glass slide.
C)relies on arrays that contain a detectable tag.
D)uses nucleic acid hybridization.
E)may use many DNA fragments that function like probes,attaches nucleotides to a solid support such as a glass slide,AND uses nucleic acid hybridization.

A)viruses.
B)bacteria.
C)plant cells.
D)animal cells.

A)high temperature.
B)high pH.
C)low temperature.
D)low salt.
E)high temperature AND high pH.

A)are useful in nucleic acid sequencing.
B)have two additional hydroxyl groups at the 2' and 3' carbons.
C)act as chain initiators.
D)act as chain terminators.
E)are useful in nucleic acid sequencing AND act as chain terminators.

A)may be obtained from denatured tagged dsDNA.
B)may be obtained from similar genes from another organism.
C)may be synthesized usually using information based on the protein sequence.
D)are usually tagged dsRNA.
E)may be obtained from denatured tagged dsDNA,may be obtained from similar genes from another organism,AND may be synthesized usually using information based on the protein sequence.

A)Escherichia
B)Bacillus
C)Pseudomonas
D)Agrobacterium

A)use the DNA directly.
B)use the DNA after it has been processed.
C)use different promoters.
D)turn mRNA into cDNA.
E)use the DNA directly AND use the DNA after it has been processed.

A)amplify certain sections of DNA.
B)amplify mRNA.
C)produce proteins.
D)produce long polymers of carbohydrates to be used in electrophoresis.

A)identifying genetic alterations associated with disease.
B)studying evolutionary relationships.
C)determining protein sequences.
D)All of the choices are correct.

A)uses virus hosts.
B)uses a labeled probe.
C)is useful in microbial ecology.
D)allows identification of particular bacterial groups in mixed samples.
E)uses a labeled probe,is useful in microbial ecology,AND allows identification of particular bacterial groups in mixed samples.

A)Nothing-it's not necessary to wash off the unbound probe.
B)You would get false-positive results in different areas where the probe hadn't actually bound,but it was still sitting there and lighting up.
C)Your FISH would be floating at the top of the tank due to the toxicity of the probe building up within them.
D)Nothing-the target nucleotide sequences are labeled,not the probe.Therefore,excess unbound probe wouldn't matter for the experiment.

A)BamHI to cut both sides-since it cuts asymmetrically,it'll leave the sticky,cohesive single-strand DNA ends that will make it easier to ligate into a BamHI-cut plasmid DNA sequence.
B)AluI to cut both sides-it's always easier to ligate together blunt ends of DNA.She should also use AluI on the plasmid she wants to put the fragment into.
C)BamHI on the fragment,and AluI on the plasmid-this will give her the matching sequences to anneal/ligate together on the fragment/plasmid combination.
D)BamHI on one side of the fragment,and AluI on the other side-this would keep the fragment from sticking right back to where it was cut out from in the original DNA.

A)Yes-you can't perform PCR without two specific primers to amplify the region in question in the DNA.
B)No-dideoxynucleotide sequencing depends on different length fragments being formed and then separated based on size.This can take place with only a specific forward OR a specific reverse primer.
C)No-you actually need a primer pair for each round of DNA amplification ...so you'll need many,many primer pairs.
D)Yes-and it will be important to make sure that the primer pairs are made with dideoxynucleotides that are labeled with fluorescent dyes.Otherwise,you won't be able to detect the fragments that are made in the PCR process.

A)Every human genome is different enough that knowing ONE human's DNA sequence can't tell us almost anything about ALL humans.
B)It's not the DNA sequence that matters-we need to know the mRNA sequence of the human genome.
C)Due to the presence of introns/exons,and splicing of RNA after transcription,the DNA sequence doesn't necessarily tell us the exact number/type of proteins that will eventually be made from it.
D)The amount of "junk DNA" present in the human genome masks any useful genetic information that we'd like to obtain.