Exam 4: lecture 13

Question 1

functions of signal-recognition particle

Answer 1

1. binding to the signal peptides
   2.blocking translation
   3.binding to the SRP receptor on the ER membrane

Question 2

how does SRP help import polypeptide into ER lumen

Answer 2

1. SRP binds to ER signal sequence (nascent polypeptide) + blocks translation
2. SRP binds to the SRP receptor; ribosome docks on membrane
3. GTP binds to SRP receptor, and newly forming polypeptide moves into pore
4. GTP is hydrolyzed and SRP is released
5. polypeptide elongates and translocates into ER lumen
6. polypeptide is completed and cleaved by signal peptidase, releasing it from the membrane

Question 3

prokaryotic gene regulation: regulated genes

Answer 3

-controlled gene, can be turned on/off when needed
*control cell growth and cell division
*expressiom is regulated by the needed of the cells and the environment as needed (not continuously)

Question 4

prokaryotic gene regulation: constitutive gene

Answer 4

-“on” all the time
*continuously expresse d
*housekeeping genes (those required for protein synthesis and glucose metabolism)

Question 5

how does transcription regulation happen

Answer 5

by controlling the access of the RNA polymerase to the promoter
(controlled whether mRNA is made or not)

Question 6

Transcriptional Regulation: Negative regulation

Answer 6

-inhibitor/repressor being made such as protein factor
-gene is ON unless a protein binds to turn it OFF
-regulatory protein turn gene OFF
-common in bacteria (can be off/on)

ex. the inhibitor blocks DNA polymerase from transcribing

Question 7

Transcriptional Regulation:Positive regulation

Answer 7

-activator, helps the process of transcription
-gene is OFF until a protein turns it ON
-regulatory proteins turn gene ON
-occurs in eukaryotes

ex. transcription is off until an activator bind to DNA polymerase to stabilize it

Question 8

what is Operon?

Answer 8

clusters of gene in which expression is regulated by operator-repressor protein interaction, operator region, and the promoter

contents:
promoter
repressor
operator (controlling site)
coding sequence
terminator

adjacent polycystronic closing sequences (bacteria, mtDNA) are cotranscribed to make polygenic mRNA

Question 9

Operon: Inducers

Answer 9

chemical/ environmental agent that initates transcription of an operon

Question 10

operon: induction

Answer 10

synthesis of gene product in repsonse to an inducer

Question 11

when are inducile genes r expressed

Answer 11

only when induced

Question 12

Lac Operon Fuction

Answer 12

allows cell to use lactose as a carbon and energy source break lactose into glucose and galactose

b-galactosidase: break down lactose ( the sugar binds)
transacetylase: help degrade/alter glactalose

Question 13

mutation in lacO

Answer 13

lacO occurs upstream of lacZ and lacY and affects production of proteins downstream on the same molecule

lacO is a regulatory sequence; no diffusible product is produced
if diffusible product is produce, expect permease production in absence of lactose

Question 14

mutstion in lacI

Answer 14

lacI produces a repressor protein

absense: repressor bind to the operator and inhibits synthesis of downstream proteins (no galactosidase/oermease are produced)

presence: repressor is inhibited by allolactose, and downstream protein synthesis occurs

Question 15

mutation is promoter (Plac)

Answer 15

inhibit RNA polymerase bidning and protein synthesis w/wo lactose

single mutation affect all three coding gene Z,Y,A

Question 16

how does positive control with catabolte activation in lac operon

Answer 16

-bacteria prefer glucose

glucose/no lactose low camp NO lac transcrip
no gluc/nolac high camp no lac
glucose + lactose low camp. no lac
lactose/no glucose high camp. lac tran

Question 17

Operon in e coli

Answer 17

tryptophan
the lower level of trp, it will turned on

-based on concentration, low levels of trp, will continue expression

presence of trp, the genes are tuned off=mRNA is not transcribed and proteins r not made

absence of trp in the medium, the genes are turned on=mRNA is transcribed and proteins are made

Q. Which molecule os the co-repressor?
trp

Question 18

how eukaryotic genes are regulated

Answer 18

time
location
dosages

Question 19

eukaryotic regulations takes place at these four levels

Answer 19

1.pre-transcriptional: before transcription (whether it wil start

2. transcriptional: controls whether transcription takes place
3. translational (post-transcriptional): what happens to mRNA once it is made (translated?)
4. post translational (protein regulation) whether protein cam be turned on/used

Question 20

Eukaryotic regulation: 1. pre-transcriptional

Answer 20

-structure of DNA open/close
a. DNA methylation
cytoson—-dna methyltransferase—–> 5-methylcytosine

b.deacetylation
c. chromatin structure

Question 21

1. pre-transactional: DNA methylation

Answer 21

cytoson—-dna methyltransferase—–> 5-methylcytosine

CpG: located around promoter of housekeeping genes/ around genes frequently expressed in a cell
=CG sequence is not methylated

CG sequences in INACTIVE genes ARE methylated to suppress their expression

Question 22

how are transcriptionally active chromatin regions tend to be?

Answer 22

hyperacetylated & hypomethylated

to do gene silencing:
histone deacetylases
ATP dependent chromatin remodolers

acetylation: add acetyle groups (red)
DNA methyltransferase: add methyl groups (yellow)
–> proteins open
deactylation: remove acetyle groups= proteins collapse
==>only methyl groups

+open/close conformation depend on availability

Question 23

Eukaryotic regulation: 2.transcriptional

Answer 23

a. transcriptionl factors
b.repsonse/control elements
c. transactivation
d. response elements

Question 24

2. transcriptional: factors

Answer 24

activator facor: helpstablize =+ regulation (RNA transcription is increased)

repressor : destabilze protein from the promoter =-regualtion(RNA transcription is inhibited)

how is transcription regulated by a receptor?
-act as binding proteins
-once glucocorticoid enters, it oushes Hsp90, causes 2 GR dimers to bind

Question 25

Eukaryotic regulation: 3. Translational

Answer 25

a. altenative splicing
b. mRNA stability
c.miRNA inhibition
d.alteration of translational factors

Question 26

3.Translational: alternative splicing

Answer 26

-25k genes
shuffle exons to get different DNA
ARE=AU Rich elements: found at the 3’ UTR they control whether eukaryotic mRNA will be degraded. the more ARE’s the quicker the degradation occurs

the longer the poly a tail 3’, the stable it is
1.deadenenylation: break down tail
2.Exosome: 3’-5’ decay (chew the actual actual mRNA)
3.decapping: 5’-3’ decay

Question 27

3.Translational: miRNA inhibition

Answer 27

-miRNA are encoded in loci other than their targets and cut to size by the ribonuclease Drosha
-they are transcribed by RNA polymerase II and their activation involves multi-step process
-expressed as longer hairpin molecules
+similar to siRNAs are generated by DICER
+associate with RISC (RNA-Inducing Silencing Complex)

+degree of complementarity to its target binding site that determines whether it will function as an miRNA/ siRNA
-22nt induce miRNA degradation or translational repression or both

Question 28

What happens during SOS function?

Answer 28

design to stop translation when cell is in serious conditions

inactive kinase—-> active kinase—autophosphorylated

-translation is inhibited because initiator tRNAmet does not bind to the 40s subunit

Question 29

Eukaryotic regulation: 4. post-translational

Answer 29

a. dependence on secondary effector
b. binding of protein subunits
c. chemical post translational modification

Question 30

4. post-translational: dependence on secondary effector

Answer 30

a. an example of needing a cofactor: the binding of an effector molecule such as a hormone

b. protein-protein:
the ability of the molecules that need to have a similar copy of themselves

1. bind to hormone
2. dimerized

ex. homodimer, heterodimer

c. posttranslational modification such as phosphorylation
-bind to phosphate to activate function

Question 31

method: Northern (RNA) Blot

Answer 31

1. take the DNA 5’TACGGA
2. expose to autoradiogram
   thru agarose cell
   nitrocellulose
   nylonmembrane

Question 32

method: western (protein) blot

Answer 32

SDS page gel -based on weight
drawbacks:
1. takes several days
2. need protein to be isolated
3. make antibodies

Question 33

method: RT-RCR(reverse transcriptase PCR)-PCR

Answer 33

PCR? copies a chain of DNA (vitro replication of DNA)
cycle: (30-35 times)
1. denature @ 90-95C (melt)
2.Reanneal @ 50-60C
3.Extension @ 72C replication
taq polymerase

long strands double in number w each round
exact sized increase exponentially
=2n

Question 34

problem : How can you do PCR like this, when the enzymes like DNA polymerase, are killed by temperature at 94c or above

Answer 34

Taq polyerase (from thermus aquaticus)

Question 35

what goes in the tube

Answer 35

primers (upstream & downstream)
dNTPS
taq polyerase
template DNA
buffer
water

Question 36

PCR misprimming

Answer 36

When PCR primers bind to the incorrect location and allow DNA polymerase to make copies of the wrong DNA within the sample. This can be caused by too low of an annealing temperature or poorly designed PCR primers that are complementary to repetitive DNA within the genome.

Question 37

RT-PCR

Answer 37

-uses mRNA as a template & reverse transcriptase which is an RNA polymerase
(RNA —RT—–> cDNA)—–PCR—-> lots of a specific cDNA template

allows to specifically amplify the cDNA from mRNA for cloning purposes
to determine whether that mRNA is being expressed or not

Question 38

Relative expression analysis by Real TIme RT-PCR (quantitative real time)

Answer 38

if cDNA is detected as present, then mRNA is present to be made into cDNA and amplified

the more mRNA is present, the faster it will be amplified

Question 39

DNA microarrays

Answer 39

used @ 100-1000 genes at once
-isolate mRNA
-convert to cDNA
-expose to light to activate fluorescent