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Cell Bio- Exam 1
Slide Set 1: Techniques and Tools in Cell Bio
Cell Culture/ Tissue Culture
Microscopy::
animal cell size- 10-30 micro m in size
Rich Medium::
9 essential aa
vitamins
peptide and GF (serum may be added)
neg charged solid surface to mimic extracellular matrix
Primary Cell culture ::
cells prepared directly from tissues of an organism
display diff props of organs which they were harvested from
cannot be passaged as much
cell strain:: lineage of cells originating from one initial primary cell culture
Transformed cells::
usually cells derived from tumor; cells that have undergone spontaneous genetic change
immortal cell line (not the same as cell strain)
grow to high densities
solid surface not required
con: may not accurately represent the og cells in tissue
FACS::
cell sorter
can sort millions of cells in just a few hours
cells go through opening one by one, cells with no charge go in waste tube, cells that have florescence pass through charged plates and go to corresponding sides of the collection chamber
Hybridomas::
used to produce monoclonal antibodies
monoclonal antibodies:: only can recognize a single epitope , used for covid treatment
to generate monoclonal antibodies:: inject antigen into animal, animal generates b cells to recognize antigen, myeloma cells fuse with b cells, transfer to to selective medium and find fused cells
Microscopy
Magnification
objective lens:: glass lens close to sample
projection lens:: close to eye
Resolution::
ability to distinguish btwn two obj
D= min distance btwn 2 distinguishable obj
N= refractive index
alpha= wavelength of angular aperture
Nsinalpha= NA
resolution is better= shorter wavelength= inc N= inc alpha
Bright field microscopy::
simple and inexpensive
no staining needed
live cell imaging
not clear for certain structures
there are ways to improve the limitations
Phase contrast Microscopy ::
modify the microscopy, certain components added to see edges of cells
thin layers of cells , live cells
DIC Microscopy ::
modified further , small details, 3D structures can be made
Sample Preparation
Fix:: using diff chemicals to kill/section the cell, partially permeabilizes cells
embedding and sectioning- cut into small pieces to look directly at underneath the microscope
H & E staining::
hemotoxylin- stain nucleus, base, purple
eosin- stains cytoplasm pink, acid
Fluorescence Microscopy
Fluorescent dyes/protiens- absorb light at shorter wavelength (excitation), emit light at longer wavelength (emission)
Fluorescence cell staining::
you can also co stain multiple colors to see different organelles/structures
Immunofluorescence Microscopy::
inject animal with primary antigen, harvest serum from animal that has antibodies in it, add 2nd fluorescent antibody to view
can only use dead cells
another way you can do this is by using GFP added to N term of protein to give it fluorescence without killing cell
Confocal Laser Scanning Microscopy (CLSM)::
focus on plane of thick specimen by rejecting out of focus light, helps improve clarity of images
Advanced Fluorescence Microscopy
FRET::
goal is to measure the dist btwn entities, can also detect conformation changes
when CFP gets closer, YFP emmits color
FRAP::
looks at how fast a mem protein can move from one side of the membrane to the other
label with fluorescent antibody, bleach with laser, measure how quickly they move
Ion Sensitive Fluorescent Dyes::
can measure the amt of ions in a structure, can see how ions are distributed within cells
TIRF::
observe thin region of specimen, helps you look at v thin sections very close to the surface
Super resolution Microscopy::
we can break the resolution limit, take lots of pics and combine to improve resolution
Electron Microscopy::
resolution is 2000x better than light microscope
TEM::
fix, embed, section (not live cells)
projects image on fluorescent screen
Immuno Electron Microscopy::
light fixation used, gold particles added to antibodies as electron dense marker bc they appears as dark spots under microscope
similar to light microscopy version
Scanning Electron Microscopy::
provide 3D image, scans surface and measures reflection
dead cells
reveals surface features of specimen
Perturbing Cellular Functions
RNAi::
used to suppress the expression of genes in cells by blocking transcription in specific mRNAs or degradation of specific mRNAs
Studying Macromolecules
Breaking up cells
separate organelles into pop of particles of diff density, shape, charge and size
Centrifugation::
more dense materials sink, lighter float
Magnetic Fractionation::
all the antibodies will bind to iron bc it is magnetic
Immunoaffinity Purification of organelles::
use antibodies to bind to organelles and purify them
Mass Spectrometer::
can tell us weight of particles
Slide set 2: Biomembrane structure
Biomembrane
Biomembrane Functions::
selective permeability only certain things can cross membrane
compartmentalize organelles formed to localize biochemical reactions
scaffold for biochemical activities- certain proteins can receive signals on membrane
transporting solutes- certain mem proteins can transport things
signal transduction
energy transduction
intercellular interaction
have transmem, peripheral, and lipid surface anchor protein
Lipids
amphiphilic :: have two diff properties, hydrophobic and hydrophilic
3 classes
Phosphoglycerides::
include phospholipids
unsat- double bonds
cis vs trans
sat- no double bonds
PS and PI carry neg charges→ help determine charge of membrane
inc mem fluidity
sphingolipids::
some are phosphoglycolipids, some are not
sphingomyelin
dec mem fluidity
sterols::
not phosphoglycolipids
ring structure
cholesterol::
rigid and planar
hydrophobic tail inserts into membrane and polar group will extend beyond membrane
usually cholesterol dec fluidity, but at low temps it can inc fluidity
no cholesterol would mean the membrane would be too fluid, too permeable, the mem would disintegrate
3 forms of phospholipid clusters::
liposome- has double layer membrane, used to deliver drugs
micelle- one layer membrane
bilayers
some conc can form structures, but it is v rare
Movement in the bilayer
transverse diffusion:: flip flop from one face to another, hard bc head group does not like to cross hydrophobic environment
lateral shift:: move across own face
flex :: turn around
flippase (ex to c) and floppase (c to ex) can aid in spontaneous flipping in the membrane, use ATP
Lipid rafts:: sphingolipid, cholesterol and certain proteins make up
Exoplasmic vs cytoplasmic::
cytoplasmic face- faces to cytosol in cell/ matrix
exoplasmic face- faces exterior, or intermembrane space
both alternate, the cytosolic face will face the matrix, then the exoplasmic faces will both be facing the intermembrane space, then the cytoplasmic face will be facing the cytosol
Liposomes as models
serve as models of biological membranes
can serve as impt tool in research, can carry antibodies, drugs, etc.
“synthetic vesicles”
Membrane Proteins
Integral
crosses at least part of the bilayer
can be solubilized with detergents
detergents:: long hydrophobic and hydrophilic tails, can interact with a protein to keep it dissolved into the solution that it is in (SDS, Triton)
Transmembrane::
crosses bilayer from cytosolic to exoplasmic face
lipid anchor::
protein on the surface by lipid is conjugated to protein and lipid is in the bilayer
acylation- use fatty acids and conjugation on n terminal side
prenylation- conjugation happens on c terminus side
GPI anchor- has sugar and phosphate, conjugate to membrane on c terminus, face towards exoplasmic surface
synthesized in ER
Peripheral::
less tightly associated, no lipid anchor, on surface of bilayer, can interact with negative head of lipids but cannot conjugate with them
Slide Set 3: Transmembrane Transport of ions and small molecules
Passive transport/simple diffusion
Common features of passive transport::
everything is non polar and small
O2, CO2, N2, EtOH, water and urea
Mediated Transport
Movement
electrochemical gradient- contains conc gradient and membrane potential (cyto more neg and exoplasmic side more positive)
Facilitated Transport
uniporters::
transport single molecule down conc gradient
aquaporins and glucose transporters
fast, reversible, specific, conformational change
GLUT1- glucose transporter expressed on plasma membrane of RBCs and endothelium or BB barrier, can pump one glucose at a time
aquaporin- water transport pore, transports water across membrane for water balance, arrangement inside porin prevents protons from entering
aquaporin 2- absence of it leads to diabetes, excretion of large vols of dilute urine
Ion channels::
form hydrophilic tube that ions can move down conc gradient
facilitated diffusion
faster than uniporters
Na/K- inside cell is negative, charge accumulates on sides. Both go from high to low conc. K moved to inside cell, Na to outside of cell , the K channel is an ion channel, Na/K pump is ATPase
patch clamping - can use small needle to clamp onto membrane and suck part of the membrane with the channel in, we can measure current flow with this technique
Active transport
ATP powered pumps::
move molecule from low conc to high conc using ATP hydrolysis
p class pumps
in plasma membrane of plants, fungi (H+ pump), and eukaryotes (Na+/K+ pump and Ca pump)
V class proton pumps
seen in many mems, almost only transport protons, couple ATP hydrolysis to transport protons against conc gradient
F class proton pumps
seen in bacterial plasma mems, almost only transport protons, utilize energy in proton concentration or voltage gradient to synthesize ATP
ABC superfam
seen in bacterial and mammalian plasma mems, have 2 transmem domains and 2 cytosolic domains that couple ATP hydrolysis to solute mvmt, switch conformation and move from one side of mem to other
symporters::
move one molecule from low conc to high conc and another from high to low, molecules moved to same side
conformational change
Na/Glucose symporter
antiporters::
move one molecule from low conc to high conc and another from high to low, opp directions
In systemic capps- Cl/HCO3 antiporter- CO2 enters cell via passive diffusion and will react to form HCO3, H2O also is involved and H is used to bind to histadine and will form hemoglobin O2 molecule. HCO3 out, Cl in, HB out
^^ can be backwards in pulmonary capps- HCO3 in, Cl out, HB in so that CO2 can leave
Bulk movement
vesicular transport::
Pinocytosis- small nutrients taken up by the cell, fluid droplets
Phagocytosis- large obj taken up by cell, bacteria
exocytosis- secretion of obj out of cell
transcellular transport::
glucose from lumen to blood
Na K ATPase- uses ATP to move Na and K from low to high conc
Na Glucose Symporter- uses Na and mem potential to pump glucose and Na from low to high conc
GLUT2- glucose uniporter
acidification of stomach lumen
combined action of 4 diff transport proteins acidifies stomach lumen while maintaining nuetral pH of cytosol
H K ATPase
K channel
Cl HCO3 antiporter
Cl channel
Slide set 4: Moving Proteins into Membranes and Organelles
Eukaryotic Protein Trafficking
Ribsomes
mem bound :: attached to cytoplasmic face of ER, synthesize secretory proteins
free ribosomes:: free in cytosol, synthesizes non secretory proteins
polyribosome :: mRNA molecule to which ribosomes are attached and engaged in protein synthesis
Secretory pathway (ER ribosomes)
secreted proteins, many plasma membrane proteins, resident proteins of secretory pathway
Steps of secretory pathway ::
import into ER
folding and glycosylation in ER
vesicular transport from ER to golgi
modifications in golgi
vesicular trafficking to final destination: plasma membrane, lysosome, endosome
Signal hypothesis::
signal sequence at n term of proteins destined for import into ER
signal seq bound by signal recognition particle (SRP)
SRP binds to GTP which is bound to the translocon
translocon translocates protein into ER
GTP released
signal peptidase cleaves off signal seq
Co translational translocation::
signal peptidase cleaves signal seq
proteins cont into lumen of ER
protein folds in Er, ribosomes detaches and floats off to being process again
Post translation translocation::
no ribosomes is bound to protein, peptide chain goes through translocon
BiP protein binds to Sec63 complex and hydrolyzes ATP
ADP cont to bind to protein along the chain and the ADP remade into ATP
Microsomes::
homogenized rough ER and smooth ER, makes vesicle like structure from pieces of ER
can show us that translation and translocation can occur simultaneously
SRP structure::
methionine residues that bind to signal seq on P54
ER membrane proteins
Type 1 ER mem proteins::
n term faces to lumen, c term to cytosol
translate until there is a stop transport anchor seq- translocation stops, translating continues
protein synthesis cont, but translocon is closed and the synthesis continues just in the cytosol
ribosome leaves, protein seq left embedded in mem
Type 2 ER mem proteins ::
n term faces cytosol instead
signal anchor seq- stops translocation into cytosol, translocation into lumen commences and transcription is cont
Type 3 ER mem proteins ::
n term faces lumen, c term cytosol
protein synthesized through translocon until signal anchor seq
translocon closes, transcription cont in cytosol
basically same as type 1 except C term tail is long here instead of n term tail being long
Type 4 ER mem proteins ::
multiple transmembrane domains
4A- n term faces cytosol
4B- n term faces lumen
GPI anchor protein ::
hydrophobic c term
ATP binds to c term
ATP binds to GET proteins
ATP hydrolyzes to transfer c term into ER mem
ATP synthesized
Hydropathy::
how to tell if proteins are transmembrane proteins
give individuals diff numbers, hydrophilic gets neg numbers, hydrophobic gets positive numbers
Resident Er proteins assist in Folding and Glycosylation in the ER
Binding protein (BiP)::
assists in post translational translocation
Protein Disulfide Isomerase (PDI)::
catalyzes the formation and rearragement of disulfide bonds (key for proper folding, function, and stability )
Glycosyltransferases::
N linked
carb chains attached to the amide nitrogen of asparagine called n linked
variable
involved in glycosylation
there is a signal for addition, quality control, folding of protein
O linked
carb chains attached to hydroxyl in serine and theronine residues
Organellar Targeting (Free ribosomes)::
nuclear proteins, mitochondrial proteins, chloroplast proteins, peroxisomal proteins, some plasma mem proteins
protein residents of other organells are directly targeted to those organelles independent of secretory pathway functions
most translated on free ribosomes
may or may not fold in cytosol
post translationally targeted into organelle
Mitochondria
Mito Encoded::
transcribed in the mito
translated on intro mito ribosomes
Nuclear Encoded::
most mito proteins
transcribed in nucleus
translated in cyto
imported into mito
Mito Import machinery::
Requires:
Import receptor- reads mito targeting signal, delivers to translocon
Translocon of outer mem- associates with import receptor, delivers protein to 2nd translocon
Translocon of Inner membrane- aligned with TOM
Matrix in Hsc70 (acts like BiP)- aids in net translocation
Path A and B
contain an N term matrix targeting seq that is recognized by the Tom 20/22 import receptor in outer mem. Only diff is that the entire precursor protein enters the matrix and is then redirected to the inner mem in path b
Path C
contain internal seq that are recognized by the Tom 70/22 import receptor , Tim 22/54 is also used
Peroxisome::
nuclear encoded
post translationally imported into peroxisome
imported as folded proteins
two targeting seq, PTS1 and PTS2
Pex5 is receptor, binds to Pex14, transfers to Pex12/2, then Pex5 releases
Nucleus::
all proteins translated in cytosol
folded proteins transported
nuclear localization signal for nuclear proteins, near c term
nuclear pore complex- spans both bilayers, huge
nuclear import- occurs via diffusion
nuclear export- driven by Ran GTPase
Ran Independent nuclear import also exists