BIOL 3416 Genetics (HW 20)
Which of the following are limitations of using restriction enzymes for the construction of recombinant DNA molecules?
- When connecting three or more DNA fragments, it is difficult to control the order in which those fragments will be connected to each other. - The researcher cannot control the directionality of the hydrogen-bonding process.
Order the following steps in cloning a gene, putting the first step at the top.
1. Chromosomal DNA is isolated and cut with a restriction enzyme 2. Digest chromosomal DNA and plasmid DNA are incubated together 3. Ligation by DNA ligase
Order the steps in one cycle of a PCR reaction, putting the first step at the top. Instructions
1. Denaturation 2. Primer annealing 3. Primer extension
In PCR, each cycle uses the products of the previous cycle as templates. What do you call this?
A chain reaction
What is a DNA library?
A collection of recombinant vectors
In gene cloning, what is the vector?
A small DNA molecule that can replicate independently within a host cell
What is a plasmid?
A small circular DNA molecule often used as a vector in gene cloning
What type of apparatus does one need to determine the amount of DNA produced during quantitative PCR?
A thermocycler that can detect fluorescence
How is the amount of DNA produced during quantitative PCR measured?
By measuring the fluorescence emitted by the probe added to the PCR mixture
In PCR, the two primers bind to specific sites in the ___ and flank the gene to be amplified.
DNA
A researcher may use restriction enzymes to digest the DNA of an organism. The fragments of DNA are then ligated individually into many vectors. This collection of recombinant vectors is called a
DNA library
Dideoxy sequencing was formulated based on scientists' knowledge of what process?
DNA replication
This technique enables researchers to determine the DNA bases in genes and other chromosomal regions.
DNA sequencing
In PCR, the template DNA is
DNA to be amplified
How is ethidium bromide used to analyze amplification by PCR?
Ethidium bromide stains DNA, allowing the size of a fragment in a gel to be determined.
In gene cloning, how is a suitable vector chosen?
It must replicate in the appropriate cell type
Which scientist developed the polymerase chain reaction?
Kary Mullis
This technique is used to identify a specific RNA molecule within a mixture of RNA molecules.
Northern blotting
What do you call the DNA sequence in a vector that allows the replication enzymes of the cell to make lots of copies of the vector?
Origin of replication
How can PCR amplify one segment of DNA from a complex mixture of potential template molecules?
Primers can be designed to flank a specific segment of DNA.
A technique used to determine the order of the nucleotides in DNA is called DNA
Quantitative PCR
You have a piece of RNA, and you want to synthesize a complementary strand of DNA. Which enzyme would you use?
Reverse transcriptase
What is recombinant DNA technology?
The production of new arrangements of DNA
When cloning a gene, why must the chromosomal DNA and the plasmid DNA be cut with the same restriction enzyme?
The sticky ends of the plasmid DNA will be complementary to the sticky ends of the chromosomal DNA.
In PCR, why do the primers bind to specific sites in the DNA on either side of the gene of interest?
They are complementary to the flanking sequences.
What is the purpose of Northern blotting?
To identify a specific RNA molecule within a mixture of RNA molecules
What is the purpose of gene cloning?
To produce many copies of a DNA molecule of interest
What technique is used to identify a particular protein in a mixture of proteins?
Western blotting
You wish to determine if a protein is made at a particular stage of development. What technique would you use?
Western blotting
The purpose of vector DNA is to
act as a carrier of a DNA sequence that is to be cloned
A particular gene to be cloned is often isolated from
chromosomal DNA
To make many copies of a gene, you would ___ that gene
clone
In PCR, primer extension refers to the synthesis of ___ starting at the primers
complementary DNA
A recombinant vector
contains a piece of chromosomal DNA
A vector requires an origin of replication so that it can be
copied many times by the host cell
Restriction endonucleases are used in gene cloning to
cut the DNA backbone prior to inserting the DNA to be cloned
In a PCR cycle, the first step is to treat the template DNA with heat, causing the strands to separate, a process called
denaturation
Reverse transcriptase PCR can be used to
detect and quantify the amount of a specific RNA.
The DNA sequencing method developed by Frederick Sanger that became a commonly used method of DNA sequencing is called
dideoxy sequencing
T/F. As long as all of the fragments have been generated using the same restriction enzyme, researchers can control the order in which three or more DNA fragments will connect to each other.
false
When using PCR to amplify DNA, short oligonucleotides called primers
flank the region of DNA to be amplified
In automated sequencing, each dideoxyribonucleotide is labeled with a different-colored
fluorescent dye
A cell that harbors a vector is called a(n)
host cell
What is the term that describes a cell that contains a DNA cloning vector?
host cell
A technique used to measure gene expression is RT-qPCR, which can determine how much ___ from a specific gene was in the original sample.
mRNA
In the technique called RT-qPCR, the starting material is
mRNA that has been reverse transcribed into DNA
A vector must contain the ___ ___ ___ that is recognized by the species of the host cell and allows the host cell to make lots of copies of the vector
origin of replication
A small DNA molecule that can replicate independently within a host cell and thus make many copies of an inserted gene is called a(n)
plasmid
A small circular DNA molecule that is often used as a vector in gene cloning is called a(n)
plasmid
In 1985, Kary Mullis developed a way to copy DNA without vectors or host cells. This technique is called
polymerase chain reaction (PCR)
During PCR, the process of ___ ___ results when the Taq polymerase catalyzes the synthesis of complementary DNA, starting at the primers.
primer extension
Short oligonucleotides that flank the region of DNA to be amplified by PCR are called
primers
The polymerase chain reaction (PCR) produces many copies of the region between two ___ that bind to sequences flanking the gene of interest.
primers
The amount of PCR product made during a quantitative PCR reaction (qPCR or RT-qPCR) is detected by changes in the level of fluorescence emitted from ___ that are added to the PCR mixture.
probes
PCR is called a chain reaction because the newly made DNA strands, or ___, of each previous reaction are used as ___ in subsequent reactions.
products reactants
The method that allows researchers to assess the amount of DNA produced during a PCR amplification as it is happening is called
quantitative PCR
The use of in vitro molecular techniques that combine DNA fragments to produce novel arrangements is called ___ DNA technology
recombinant
A vector that contains a piece of chromosomal DNA is referred to as a(n)
recombinant vector
Enzymes that bind to a specific DNA sequence and cut the DNA backbone are called
restriction enzymes
The enzyme that uses RNA as a template to make a complementary strand of DNA is called
reverse transcriptase
The use of dideoxyribonucleotides with different-colored fluorescent dyes allows the detection of the
sequence of DNA
Primer annealing occurs when
short oligonucleotides bind to complementary DNA flanking the gene of interest
In PCR, the DNA to be amplified is called the
template DNA
T/F. Chromosomal DNA is a common source of cloned DNA.
true
T/F. PCR can amplify one segment of DNA from a mixture.
true
A DNA molecule that acts as a carrier of DNA that is to be cloned is called a(n)
vector