Exam 2 T/F AGR3303
The tumor inducing (Ti) plasmid in soil bacteria can be moved and replaced by your gene of interest for plant transformation
true
Ti plasmid can be modified or engineered as a vector for plant transformation
true
The Illumina sequencing has a much higher throughput than Sanger sequencing method
True Throughput - number of sequencing reactions to be done simultaneously in one run in sequences
insertion or removal of one or more nucleotide base pairs in a gene usually results in a frame shift mutation
true
siRNA in RITS binds to DNA and causes methylation, restricting transcription
True
GAL4 is a transcription repressor for the galactose-digesting enzyme gene
False GAL4 is an activator
The lengths of reads from Illumina sequencing method is much longer than the reads from Sanger method
False Length of reads from Sanger are much longer, Illumina is normally 50-150bp and up to 300bp while Sanger is 500-800bp
RITS consists of miRNA
False RITS consist of siRNAs and proteins the siRNA in RITS binds to DNA and causes methylation -> restricts transcription
Restriction enzymes randomly cut dsDNA and produce either cohesive or blunt ends
False Restriction enzymes recognize specific nucleotide sequences (4-8 base pairs long) to cut dsDNA (double stranded DNA)
Illlumina sequencing is more advanced than Sanger sequencing method, which makes Sanger sequencing method lost its value
False Sanger is still gold standard
A missense mutation changes a codon that specifies an amino acid into one that terminates translation
False a missense mutation is a base substitution that results in a different aa a nonsense mutation is a substitution that changes a sense codon into a stop codon
Addition of acetyl groups to the tails of histone proteins usually results in repression of transcription, FLD deacetylates histones that bind to regions of FLC gene and stimulates its transcription
False addition of acetyl groups (acetylation) of histone proteins weakens their interaction w/ DNA and allows transcription factors to bind to DNA, increasing transcription
Nonsense mutations do not alter the amino acid sequence chain
False change sense codon (for an aa) into a stop codon
During gene cloning, the vector DNA sequence with foreign DNA will integrate into the host DNA. When the host cell divides, copies of the recombinant DNA molecules are passed to the progeny
False cloning vector carries the foreign DNA piece (recombinant DNA) independent of the bacterial host DNA
In the absence of allolactose, the lac operon is constitutively transcribed
False constitutively transcribed - always being transcribed when allolactose or lactose is present, genes are expressed to metabolize lactose (negative inductable)
A repressible gene should be under control by a repressor
False regulator protein can be repressors (negative control, inhibits transcription) or activators (positive control, stimulates transcription) these can be inducible operons (transcription normally off) or repressible operons(transcription normally on)
Taq polymerase enzyme, used for PCR, denatures at 94C
False the Taq polymerase can tolerate this temp while DNA denatures into single strands
In the absence of tryptophan, the genes of the trp operon for tryptophan synthesis are not expressed
False they are expressed, then tryptophan is present it binds to the repressor and makes it active which binds to the operator which shuts off transcription (negative repressible)
A mutation that changes G/C base pair to A/T is a transversion mutation
False A=T G=_C Transition (common) - like to like (purine->purine) Transversion -like to unlike (purine -> pyrimidine)
Agarose-gel electrophoresis can be used to separate DNA or RNA molecules only on the basis of their electrical charge
False Agarose gel electrophoresis uses both electrical change and size to separate DNA/RNA molecules
In eukaryotes, most structural genes are found within operons
False In most prokaryotes, structural genes are found within operons
PCR has three recurring steps: denature, primer annealing, and hybridization
False PCR (polymerase chain reaction) 3 steps are denaturing, primer annealing, and primer extension
Plasmid is a small circular DNA and thousands of of base pairs with functional genes but does not have its own origin of replication
False Plasmids have an ori (origin of replication)
Somatic mutation are not transmitted to new daughter cells
False Somatic mutations are passed to daughter cells
When siRNAs are present, the rate of its target mRNA degradation decreases and the rate of protein production increases
False Targeted mRNA degradation increases and protein production decreases How it works: siRNA pairs with protein to form RISC (RNA-induced silencing complex) -> siRNA in RISCs pair w/ mRNA and cleaves it -> mRNA is degraded, broken down, and amount of protein is decreased
Illumina sequencing is a method of sequencing by synthesis, which relies on incorporation of nucleotides with an irreversible terminating group by a DNA polymerase
False The nucleotides in Illumina sequencing have reversible terminating groups
Base analogs are mutagenic because they distort the structure of DNA
False base analogs cause the base to change (base substitution)
During RNA interference, miRNA in RISCs match the mRNA imperfectly and stimulate the translation of targeted mRNA
False miRNA matching up imperfectly inhibits translation of targeted mRNA
in a bacterial operon, promoter is bound by regulator protein to regulate its transcription
False the promoter is bound by RNA polymerase the regulator protein is encoded within the promoter (can be active/inactive)
After gene cloning, bacteria with 'empty' or no insert plasmids are blue because they have a functional lacZ. so we are not selecting the blue colony for the cloned gene
True bacteria with the inserted gene have nonfunction lacZ and are white
An expression vector is needed for GMO
True ensures transcription and translation cloning vectors - carry recombinant DNA
Lac operon has both negative and postive controls
True regulatory proteins negative control - repressor, represses transcription positive control - activator, stimulates transcription
During DNA replication, incorporation of 5-Bromouracil can lead to transition mutation
True 5-BU is a base analog (has BR atom) for thymine
DNA fragment clusters are generated for optical detector in the Illumina sequencer to be able to detect string enough signal during sequencing
True
During RNA interference for cleavage of mRNA, siRNA in RISC pairs with mRNA and RISC cleaves the mRNA
True
For a gene under negative control, the regulator protein is a repressor
True
For a gene under positive inducible control, regulator protein is an activator and normally the gene is inactive in transcription
True
RNA interference is also known as RNA silencing and posttranscriptional gene silencing
True
The rate of degradation of mRNAs is important in gene regulation in eukaryotes
True
During Sanger sequencing, the incorporation of a deoxynucleotide terminates DNA synthesis because it lack 3'OH
false dideoxynucleotide terminates DNA synthesis because it has an H at 3'C (lack OH to create phosphodiester bond w/ next nucleotide)
A cloning vector has three important characteristics: 1. origin of replication 2. selectable marker 3. unique restriction enzyme sites
true
DNA replication errors cause spontaneous mutations
true
In a general sense, highly condensed DNA bound with histone proteins represses gene expression
true
Regulatory genes are genes whose products control the transcription or translation of other genes
true
Alternative splicing is known to be important in the regulation of the sexual development in Drosophila
true determines male/female
UV light can be absorbed by pyrimidine in DNA resulting in pyrimidine dimers
true pyrimidine dimers are a chemically bonded adjacent pyrimidines on a DNA strand, often block DNA replication which inhibits cell division
transposition can cause gene mutation
true transposition - the movement of TE (transposable elements /transposons- DNA sequences capable of moving positions in the genome) from one location to another in the genome facilitated by transposase
