Bacterial Genetics
match the analytic method with the description
* DNA fingerprinting/profiling = demonstrates unique patterns of DNA fragments in a gel. * polymerase chain reaction(PCR) = amplifies a specific DNA sequence so that there are enough coples that they can be readily detected if present. * DNA sequencing = determines the order of nitrogenous bases in DNA. * DNA probes = detects specific short DNA sequences characteristic of a specific microorganism
match each of the items needed for PCR with their function in the reaction
* template DNA strand = provides the target sequence which will be amplified * primers = direct the DNA polymerase to the target sequence and provide starting material for DNA polymerase to add on to * thermostable polymerase = synthesize new DNA strands * thermocycler = controls and quickly modifies the reaction temperature as needed * free deoxynucleotides = building block that are added to form the new DNA strands
match the inoculated agar plates with their expected growth after incubation
-pGLO on LB = very dense white bacterial growth +pGLO on LB/amp = white bacterial colonies -pGLO on LB/amp = no growth +pGLO on LB/amp/ara = green fluorescent bacterial colonies
place the steps of one PCR cycle into the correct order
1. denaturation 2. priming 3. extension
the following steps are completed when preparing a sample for PCR. place the steps in the correct order
1. label microcentrifuge tubes 2. add DNA samples to microcentrifuge tubes using a new micropipet tip for each sample 3. add prepared master mix containing Taq polymerase, primers, deoxynucleotides, and buffer to microcentrifuge tubes 4. place PCR tubes into thermocycler, set program, and start
order the following general steps of a transformation exercise
1. label two tubes as +pGLO and -pGLO 2. add bacteria to +pGLO and -pGLO tubes 3. add plasmid to the +pGLO tube only 4. move the -pGLO and +pGLO tubes from ice to water bath 5. move the -pGLO and +pGLO tubes from the water bath to ice 6. add LB broth to both tubes 7. inoculate plates of LB, LB/amp, and LB/amp/ara agar as labeled
how should PCR products be stored after completion of PCR, prior to gel electrophoresis
4C
which of the following best portrays the direction of genetic information flow, according to the central dogma of biology
DNA -> RNA -> Protein
which of the following are correctly paired
GFP gene--fluorescent green protein bla gene--ampicillin resistance
match the type of medium with its description
LB agar = nonselective medium for bacteria LB/amp agar = selective medium containing an antibiotic to inhibit the growth of nonresistant cells LB/amp/ara agar = selective medium with added antibiotic and sugar to select for transformants and allow full plasmid expression
which of the following is accomplished by use of PCR
a specific sequence of DNA can be amplified a billion fold
indicate the four nitrogenous bases that are found in DNA
adenine, guanine, cytosine, thymine
which of the following are correct steps in transformation process
bacteria is added to both +pGLO and -pGLO tubes; move the -pGLO and +pGLO tubes from ice to water bath to ice
primers provide the specific location where DNA synthesis will ___
begin
where should the micropipet tip be when delivering a DNA specimen into a well in an agarose gel
below the buffer surface, in the upper portion of the well
which of the following are needed to cast the agarose gel
comb, liquefied agarose, gel tray
the bonds that join the nucleotides in DNA to form the sugar-phosphate backbone are ___ bonds
covalent
which of the following are included in the master mix used to perform PCR
deoxynucleotides primers buffer taq polymerase
select the three components of a nucleotide in DNA
deoxyribose, nitrogenous base, phosphate
which of the following are potential applications of PCR
detection of DNA during crime scene analysis. detection and identification of infectious agents in patient samples. detection of DNA from victims of massive disasters.
which of the following is used to stain the DNA in a gel for viewing after electrophoresis
ethidium bromide
a single nucleotide change in a DNA sequence is not enough to alter any protein structure in an organism
false
all RNA molecules serve as templates for protein synthesis
false
all mutations result in phenotypic change in an organism
false
indicate the items needed for PCR
free deoxynucleotides thermostable DNA polymerase primers template DNA with target sequence
which of the following can be used to detect the products of PCR
gel electrophoresis
the deliberate manipulation of an organism's genome in the laboratory is specifically known as ___
genetic engineering
human genes can be introduced into bacterial cells via transformation, after which the bacteria cells express the human gene, producing a human protein such as insulin or growth hormone. the bacterial cell is described as ___
genetically-modified, a recombinant cell
how is the agarose prepared prior to pouring the gel
it is dissolved into buffer by heating
how can you recognize a transformed bacterial cell from a non transformed bacterial cell
it will grow on agar with added ampicillin and may appear green
what is mixed the PCR samples just prior to loading them into the gel for electrophoresis
loading dye
a single nucleotide change in the original sequence of DNA is a ___
mutation
when positioning the gel in the electrophoresis chamber, the wells should be closet to the ___ electrode
negative
following PCR, the products were loaded into a gel and electrophoresis was performed. following staining of the gel, no band of DNA was observed. based on this observation, was the desired sequence successfully amplified
no
the progress of the DNA fragments through the gel can be monitored by ___
observing the movement of the bromophenol blue loading dye
when a gene of interest from one organism is introduced into a plasmid, the plasmid is referred to as a ___ plasmid
recombinant
plasmids used as cloning vectors often include a gene for antibiotic resistance, this makes it easier to isolate bacterial cells that have been successfully transformed with the plasmid by using a medium containing the same antibiotic. such an antibiotic-containing medium would be described as ___
selective
match the reagents used in the master mix with their purpose in the polymerase chain reaction
taq polymerase = heat-stable enzyme that builds the new DNA molecules dNTP mixture = free nucleotides used to build the new DNA molecules primers = short DNA sequences that direct the synthesis of the target DNA buffer = a reagent used to enhance the activity of enzymes in the mixture
primers selected for PCR must hybridize with ___
the DNA flanking either end of the target sequence
why is the bacterial growth white when +pGLO is plated onto LB/amp agar
the cells cannot transcribe the GFP gene without the presence of arabinose
if arabinose was accidentally left out of the LB/amp/ara plates, what would happen when +pGLO cells were plated on the medium
the cells would be white instead of green/fluorescent
in which of the following ways does the gene for sickle cell hemoglobin differ from the gene for normal hemoglobin
there is a single nucleotide difference
what would be the consequence of not including a lane with the DNA ladder on an electrophoresis gel
there would be no way to determine the size of the fragments
what is the purpose of the -pGLO on LB/amp plate
this plate can be compared to the -pGLO on LB agar plate to show that the cells are not naturally resistant to ampicillin this plate can be compared to the +pGLO on LB/amp plate to show that transformation confers
the process of copying a strand of DNA to form a strand of RNA is called
transcription
genes for human growth hormone and for human insulin have been placed into plasmids and introduced into bacteria by means of ___
transformation
the process by which a bacterial cell picks up small pieces of DNA from the surrounding environment is referred to as
transformation
E. coli cells are made competent for transformation by ___ and ___
treating them with calcium chloride; subjecting them to a brief heat shock
UV illumination is necessary to view ethidium bromide-stained DNA in an electrophoresis gel
true
different species of microorganisms as well as different strains within a species can usually be distinguished by genetic differences
true
if growth appears on the LB/amp plate labeled as -pGLO, what might explain this unexpected result
you accidentally inoculated the plate from the +pGLO tube the ampicillin is actually missing from the medium the original bacterial cells were naturally resistant to ampicillin
how would you explain a lack of expected growth on the control -pGLO/LB plate
you forgot to add bacterial cells to the -pGLO tube
