Post on 10-May-2015
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Proteins – Basics you need to know for Proteomics
Outline for Rest of Course• Proteins and Exploring Proteins
– Basics of protein structure– Basics of conventional protein analysis
• PTMs of Proteins (Walsh)– Phosphorylation– Glycosylation
• Intro to Proteomics (Simpson, Ch 1)• HPLC (Simpson, Ch 5)
– RP-HPLC– 2D-HPLC– Lab Demo of nano-HPLC
• Peptide Mapping (Simpson, Ch. 7)– Lab demo
• Mass Spectrometry (Simpson, Ch.8)– Ionization – ESI, MALDI– Separation – TOF, Quad, IT, FT-ICR– Tandem MS– Fragmentation (p 577, and Mascot tutorial)– Lab demos– Bioinformatics for Proteomics
Objectives
• Understand basics of protein composition and structure
• 20 naturally occurring amino acids and their properties
• Secondary structural motifs
• Tertiary and Quaternary structure
• Protein synthesis
• Basic biochemistry techniques
Protein Structure and Function
• Functions– Enzymes – catalysts of chemical reactions– Transport and storage – Fe, O2, CO2, Cu, etc.– Motion and motors – muscles, flagella– Structural support – collagen, elastase, actin– Immune protection – antibodies, cytokines– Stimuli response – vision, touch, smell, taste– Growth and differentiation – growth factors,
hormones, cytokines
Aliphatic side chains
(hydrophobic)
Proline
• Imino acid• Side chain bound to -carbon and N• Often found in bends of protein chains• Unique properties (more later)
Aromatic Side Chains
• Very hydrophobic• Tyr – OH is reactive• Absorbance at 280 nm
Sulfur Containing AA’s – Met, Cys
• Cys sulfur is highly reactive– Reduction/oxidation– Protein folding
• Hydrophobic
Disulfide Bonds - CysReduced Oxidized
Remember: LEO says GER
Hydroxyl side groups – Ser, Thr
• More hydrophilic• Ser OH group can
be reactive (serine proteases)
• Lys and Arg are (+) at pH 7• His can be
protonated/deprotonated
Polar side groups - basic
Polar side groups - acidic
• Negatively charged at pH >6
Polar side groups - neutral
• Terminal amide groups
• Can be de-amidated to Glu and Asp
Ionizable AA’s
• pKa values must be memorized
• pKa values are highly dependent on local environment
Polypeptides• Mnemonic: NCC-NCC-NCC-NCC• Always given with amino terminus (N-terminus) at
beginning
• 1 Dalton = 1 amu• Avg MW of aa is ~110 Da
Post-translational Modifications of AA’s
• Some aa’s are chemically modified after protein synthesis– Often used to confer special biochemical properties essential to
protein’s function– Examples
• Acetylation of N-terminus • Hydroxylation of Pro (collagen)• Carboxylation of Glu (blood coagulation enzymes)• Phosphorylation of Ser, Thr, Tyr (cytokine receptors)• Sulfation of Tyr• Glycosylation of Ser, Thr, Asn
• Proteins can also be proteolytically processed– Zymogen to active enzyme (trypsinogen/trypsin)– Fibrinogen to fibrin (to form blood clot)– Prohormones to hormones
• Lots more on this later
tRNA Molecules
• General features– 73 to 93 ribonucleotides
(25 kD)– Methylated or
dimethylated versions of bases (structure)
– Cloverleaf structure with anti-codon loop
– 5’ phosphorylated
• Amino acid at 3’
•IGC complementary to GCC (A)
3-D structure
• L-shaped molecule – anti-codon and amino acid attachment at opposite ends
• CCA – conserved sequence for amino acid attachment
• 4 helices
Ribosomes – molecular machines
• Coordinate charged tRNA’s, mRNA, and nascent polypeptides during protein synthesis
• Macromolecular complex– 50S subunit – 34 proteins + 2 RNA molecules: L1-L34; 23S
and 5S RNA – 30S subunit – 21 proteins + 1 RNA: S1-S21; 16S RNA – S20 and L26 are identical– One copy of each RNA, two copies L7 and L12, 1 copy of
all other proteins• L7 and L12 identical except L7 N-term is acetylated
• Prokaryotes - Many ribosomes can translate a single mRNA at the same time
• “Polysome” or “Polyribosome”
Tunnel for growing polypeptide chain
Protein synthesis initiation
• E. coli - Formylmethionyl tRNA– Removed from
protein after about 10 amino acids in ~50% of proteins
• Specific mechanism for f-Met synthesis and incorporation
Why Formylation of Met?
Termination of translation if not formylated!
Animated versions
• Narrated Animation – prokaryote protein synthesis– Prokaryote vs. eukaryote– Splicing– Protein secretion
Gel Filtration – molecular size
Ion exchange chromatography
+++ +Cl- Cl- Cl-Cl-
+++ +
+++ +Cl- Cl- Cl-Cl-
Affinity Chromatography
Equilibrate column
Load feed onto columnThen wash contaminants away
Elute Product
Clean Column and re-equilibrate column
Reverse Phase High Performance Liquid Chromatography - RP-HPLC• Used for both purification and as an
analytical tool
• High Resolution – able to separate proteins based on very small differences in structure
RP-HPLC Mechanism of Separation
• Stationary phase – hydrophobic groups – C4, C5, C8, C18, phenyl– Proteins are dissolved in mostly aqueous buffer and
injected onto the column– Molecules interact with the stationary phase– Organic solvent (modifier) is added to the mobile
phase and kicks the molecules off the stationary phase
Purity by HPLC
• HPLC is high resolution and can be used to assess purity of a protein sample– Compare with known
reference standard of desired protein and potential contaminants
– Can be quantitative – determine protein concentration by constructing calibration curve
Visualizing the effects of Purification - Electrophoresis
• Gel Electrophoresis can be used to visualize the effectiveness of purification and estimate protein MW
• Proteins migrate through the porous hydrogel based on molecular size – radius of gyration.
Isoelectric Focusing - IEF• IEF separates molecules based on their isoelectric
points (IEP), or the pH at which they have a net neutral charge
• IEF is usually used as an analytical tool to confirm a protein’s structure, but there are some semi-preparative devices that can be used for protein purification (difficult to run, though)
• IEF is very powerful – proteins with IEP’s that differ by as little as 0.01 pH can be separated using specialized techniques
• IEF can be run in a slab gel (similar to SDS PAGE format), in tubes, on paper strips, or in capillaries
• IEF is also used a lot in proteomics research
IEF Basics• Consider a slab gel – polyacrylamide that is impregnated with “ampholytes” • Ampholytes are a mixture of synthetic polymers (usually amino acids) that vary in their IEP, say from pH 3
to pH 10. The ampholytes are usually pre-focused (but don’t have to be) to set up a pH gradient in the gel• The samples for analysis are NOT treated with SDS or reductant – they are added to the IEF gel in their
native state with a small amount of ampholytes
pH 3
pH 10
Running an IEF Gel
pH 3
pH 10
• Samples are added to the Gel and gel is placed in apparatus. The upper chamber is filled with anolyte (10 mM phosphoric acid) and the lower chamber is filled with catholyte (20 mM NaOH). The electric field is then turned on.
upper chamber – phosphoric acid(+) positive electrode
lower chamber - NaOH(-) negative electrode
power supply
• The ampholytes and sample proteins will migrate until their charge is neutral, then they don’t migrate any more. Thus a stable pH gradient is set up, and molecules are separated based on their differences in IEP• The proteins are then stained for visualization
IEF Examples
Monoclonal Antibody Production
2-D SDS PAGE
• Two-dimensional separation– 1st dimension – IEF (paper strips, tube gels)– 2nd dimension – SDS PAGE
• Lay paper strip down on top of gel; run 2nd dimension
Immunological Assays
• Use of antibodies to detect, purify, and qunatify your protein of interest
• Antibodies– Immunoglobulins that have a high affinity for their respective
antigen
• Antigen – substance that elicits an immune response– Proteins, oligosaccharides, small organic molecules (hapten)– Epitope – structural portion of the antigen that directly interacts
with antibody
• Ab/Ag interaction ~ lock and key– NONCOVALENT – a combination of H-bonds, van der Waals,
and ionic interactions with surface topology
IgG’s
Ag/Ab interactions
ELISAs
Western Blots
Immunohistochemistry, Immunoelectron microscopy