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ACS BIOCHEMISTRY FINAL EXAM STUDY GUIDE | Actual Questions and Answers Latest Updated 2024/2025 (Graded A+)Exam (elaborations) Bio chem

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Henderson-Hasselbach Equation - pH = pKa + log ([A-] / [HA]) Salting Out (Purification) - Changes soluble protein to solid precipitate. Protein precipitates when the charges on the protein match the charges in the solution. Size-Exclusion Chromatography - Separates sample based on size with smaller molecules eluting later. Ion-Exchange Chromatography - Separates sample based on charge. CM attracts +, DEAE attracts -. May have repulsion effect on like charges. Salt or acid used to remove stuck proteins. Hydrophobic/Reverse Phase Chromatography - Beads are coated with a carbon chain. Hydrophobic proteins stick better. Elute with non-H-bonding solvent (acetonitrile). Affinity Chromatography - Attach a ligand that binds a protein to a bead. Elute with harsh chemicals or similar ligand. SDS-PAGE - Uses SDS. Gel is made from cross-linked polyacrylamide. Separates based off of mass with smaller molecules moving faster. Visualized with Coomassie blue. SDS - Sodium dodecyl sulfate. Unfolds proteins and gives them uniform negative charge. Isoelectric Focusing - Variation of gel electrophoresis where protein charge matters. Involves electrodes and pH gradient. Protein stops at their pI when neutral.

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ACS BIOCHEMISTRY FINAL EXAM STUDY GUIDE | Actual Questions
and Answers Latest Updated 2024/2025 (Graded A+)


Henderson-Hasselbach Equation - ✔✔pH = pKa + log ([A-] / [HA])



Salting Out (Purification) - ✔✔Changes soluble protein to solid precipitate. Protein precipitates when
the charges on the protein match the charges in the solution.



Size-Exclusion Chromatography - ✔✔Separates sample based on size with smaller molecules eluting
later.



Ion-Exchange Chromatography - ✔✔Separates sample based on charge. CM attracts +, DEAE attracts -.
May have repulsion effect on like charges. Salt or acid used to remove stuck proteins.



Hydrophobic/Reverse Phase Chromatography - ✔✔Beads are coated with a carbon chain. Hydrophobic
proteins stick better. Elute with non-H-bonding solvent (acetonitrile).



Affinity Chromatography - ✔✔Attach a ligand that binds a protein to a bead. Elute with harsh chemicals
or similar ligand.



SDS-PAGE - ✔✔Uses SDS. Gel is made from cross-linked polyacrylamide. Separates based off of mass
with smaller molecules moving faster. Visualized with Coomassie blue.



SDS - ✔✔Sodium dodecyl sulfate. Unfolds proteins and gives them uniform negative charge.



Isoelectric Focusing - ✔✔Variation of gel electrophoresis where protein charge matters. Involves
electrodes and pH gradient. Protein stops at their pI when neutral.



Iodoacetate - ✔✔Adds carboxymethyl group on free -SH groups. Blocks disulfide bonding.



Homologs - ✔✔Shares 25% identity with another gene

,Orthologs - ✔✔Similar genes in different organisms



Ramachandran Plot - ✔✔Shows favorable phi-psi angle combinations. 3 main "wells" for α-helices, ß-
sheets, and left-handed α-helices.



α-helices - ✔✔Ala is common, Gly & Pro are not very common. Side-chain interactions every 3 or 4
residues. Turns once every 3.6 residues. Distance between backbones is 5.4Å.



Helix Dipole - ✔✔Formed from added dipole moments of all hydrogen bonds in an α-helix. N-terminus is
δ+ and C-terminus is δ-.



ß-sheet - ✔✔Either parallel or anti-parallel. Often twisted to increase strength.



Anti-parallel ß-sheet - ✔✔Alternating sheet directions (C & N-termini don't line-up). Has straight H-
bonds.



Parallel ß-sheet - ✔✔Same sheet directions (C & N-termini line up). Has angled H-bonds.



ß-turns - ✔✔Tight u-turns with specific phi-psi angles. Must have gly at position 3. Proline may also be at
ß-turn because it can have a cis-omega angle.



Loops - ✔✔Not highly structured. Not necessary highly flexible, but can occasionally move. Very variable
in sequence.



Circular Dichroism - ✔✔Uses UV light to measure 2° structure. Can be used to measure destabilization.



Disulfide-bonds - ✔✔Bonds between two -SH groups that form between 2° and 3° structure.



ß-mercaptoethanol - ✔✔Breaks disulfide bonds.

, α-keratin - ✔✔formed from 2 α-helices twisted around each other. "Coiled coil". Cross-linked by
disulfide bonds.



Collagen - ✔✔Repeating sequence of Gly-X-Pro. 3 stranded "coiled coil". Contains gly core.



Myoglobin 4° Structure - ✔✔Symmetric homodimer,



Hemoglobin 4° Structure - ✔✔Tetramer. Dimer of dimers. α2ß2 tetramer.



Mechanism of Denaturants - ✔✔Highly soluble, H-binding molecules. Stabilize protein backbone in
water. Allows denatured state to be stabilized.



Temperature Denaturation of Protein - ✔✔Midpoint of reaction is Tm.



Cooperative Protein Folding - ✔✔Folding transition is sharp. More reversible.



Folding Funnel - ✔✔Shows 3D version of 2D energy states. Lowest energy is stable protein. Rough
funnel is less cooperative.



Protein-Protein Interfaces - ✔✔"Core" and "fringe" of the interfaces. Core is more hydrophobic and is
on the inside when interfaced. Fringe is more hydrophilic.



π-π Ring Stacking - ✔✔Weird interaction where aromatic rings stack on each other in positive
interaction.



Fe Binding of O2 - ✔✔Fe2+ binds to O2 reversible. Fe3+ has an additional + charge and binds to O2
irreversibly. Fe3+ rusts in O2 rich environments.



ϴ-value in Binding - ✔✔ϴ = (bound / total)x100%
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