Cell Bio (BI220) lab practical- Butler university
8 steps to western blot
1. sample prep 2. gel electrophoresis 3. blotting 4. blocking 5. antibody probing 6. detection 7. imaging 8. analysis
what is the enzyme that digests lactose
B-galactosidase
4 components of HeLa medium
BSA penicillin glutamine pyruvate
indicator dye to monitor ETC
DCPIP
negative control
DMSO; doesn't effect experiment
fluorescence microscope
Instrument used to visualize a specimen that has been labeled with a fluorescent dye; samples are illuminated with a wavelength of light that excites the dye, causing it to fluoresce. beneficial to see only specific compounds
kingdoms
Plants, Animals, Protists, Fungi, Archaebacteria, Eubacteria
what is control measured in
RPM
why is gravity reported
RPM changes
why is absorbance used instead of %T
absorbance directly proportional to concentration
p value greater than 0.05
accept null hypothesis; is not significant
excitation
allow light through narrow band of wavelength; excites fluorescent molecule
coomassie blue stain
allow you to see bands representing most prominent proteins in gel
control experiment
an experiment designed to control for variables affecting the results of another experiment
antibody exposure
apply detector compound to see microtubules
why must tubes in centrifuge be opposite from eachother
balance; can ruin centrifuge otherwise fragments can fly and hit walls, humans, etc
secondary antibody
binds to primary antibody
DAPI
blue stain; helps see nucleus by binding to DNA and detect apoptosis
bromophenol blue
blue tracking dye
tris
buffer
light microscope
carries information to your eye; place specimen in the path of the beam of light. Light paces through lenses, until reaches eye.
why is regular passaging needed for cell culture
cells need nutrients and room to grow
making tagged antibodies for every antigen is expensive so;
cheaper to have untagged primary antibody to recognize antigen and tagged secondary antibody to recognize all primary antibodies
positive control
colchicine; depolymerization of microtubules
what does the PBS allow in cell culture
constant pH and remove media
if something is turning clear, will the absorbance increase or decrease
decrease
SDS
detergent
2 functions of SDS detergent in SDS-PAGE
disrupt membranes and denature proteins sticks to proteins to change charge
function of heat in SDS-PAGE
disrupts all 4 types of interactions between R-groups and hydrogen bonds involved in alpha helices and beta pleated sheets (secondary)
permeabilization
dissolve cell membrane allow larger dye molecules to enter inside the cell
function of glutamine in medium
energy source
control variable
factor kept constant
why laminar flow hood
filters and sterilizes air while running
steps involved with immunoflourescence
fixation permeabilization blocking antibody exposure mounting
nucleus
genetic material
antibodies
glow green; helps see microtubules and detect apoptosis
g
gravity at sea level
function of BSA in medium
growth factors
primary antibody
has a specific target antigen
first step of differential centrifugation
heavy debri (unbroken cells and walls) separated by short, low speed spin
purpose of loading control
indicate equal loading of samples across all wells and proper transfer of proteins to membrane
sample preparation for western blot
isolate appropriate protein fraction by centrifuge proteins denatured and coated with SDS
fixation
killing cells but keeping them in life like state
standard curve x-axis
known amount
type of hood used for cell culture
laminar flow hood
western blot
looking at specific proteins (antibodies bind to specific antigens)
nucleolus
makes ribosomes
function of glycerol in SDS-PAGE
makes samples dense enough to stay in wells
what is left in supernatant after second step of differential centrifugation
membrane fragments and lower-density organelles
object of SDS-PAGE
minimize difference between proteins so electrophoretic mobility depends on molecular weight
when centrifuging, more dense compounds will
move faster and end up closer to bottom
heavier organelles
move more quickly; not needed to be spun at high speed
emission
narrows exactly what wavelengths reach your eye and camera
light organelles
need spun more quickly in order to pellet
mounting
onto slides allow visual under IFM
2 functions of DTT reducing agent in SDS-PAGE
oxidizes proteins breaks disulfide bridges into 2 separate sulfhydryl groups
environmental factors that influence enzyme function
pH temperature concentration presence of inhibitors/activators
chloroplast
photosynthesis
what does PAGE stand for
polyacrylamide gel electrophoresis
why is sucrose in chloroplast isolation buffer
prevent chloroplast from bursting
function of penicillin in medium
prevent contanimation
without DTT reducing agent
primary structure would not be linearized quaternary structure would stick together
third step of differential centrifugation
purified chloroplasts broken by osmotic shock; thylakoids pelleted away from chloroplasts
total centrifuge force depends on
quickness of rotor spins radius of rotor
DTT
reducing agent
p value less than .05
reject the null hypothesis; is significant
function of tris in SDS-PAGE
resists change of pH
RPM
revolutions per minute
2 functions of bromophenol blue in SDS-PAGE
runs faster than proteins on gel monitors progress
plasma membrane
separate cytoplasm from inside of cell
with secondary antibody
signal is stronger
why must lid be closed during centrifugation
so things don't fly and hit somebody (wait to open until done spinning)
what does SDS stand for
sodium dodecyl sulfate
function of pyruvate in medium
source of carbon and glucose
2 sections of gel with different densities
stacking and separating gel
vacuole
storage; turgor pressure
microtubules
structure/support; motor proteins; cell cycle
second step of differential centrifugation
supernatant (liquid) spun at longer and higher speed to pellet chloroplasts
transmission electron microscope
thin specimens; 2D image; all details of cytoplasm visible. con: takes a long time to process
Why are the cells incubated at 37°C?
to put the enzymes at their optimal temperature to work at
types of electron microscopes
transmission and scanning
how are the cells released
trypsin
standard curve y-axis
unknown amount (measuring)
electron microscope
uses electrons to generate an image
independent variable
variable that is manipulated
dependent variable
variable that is measured
glycerol
viscous liquid
scanning electron microscope
whole specimen; 3D image; very fine details on surface visible
