Enzyme → reads DNA template 3'→5', synthesizes RNA 5'→3' using NTPs (ATP, UTP, GTP, CTP) as substrates. No primer needed. Prok: 1 RNA pol (5 subunits: α₂ββ'ω). Euk: Pol I, II, III.

Key facts: Transcription bubble = ~12-14 bp unwound DNA. Error rate ~10⁻⁴. β subunit = catalytic site (phosphodiester bond formation), β' = DNA binding, α = assembly + UP element contacts, ω = assembly/stability

Prok initiation subunit → binds core enzyme (α₂ββ'ω) to form holoenzyme. σ⁷⁰ = primary/housekeeping factor. Region 4.2 contacts -35 (TTGACA); region 2.4 contacts -10 (TATAAT). Melts ~12 bp at -10 to form open complex.

Key facts: σ70 recognizes -10 (TATAAT) and -35 (TTGACA) elements; dissociates after ~10 nt synthesized

Bacterial RNA polymerase minus the σ subunit (α₂ββ'ω); can elongate but not initiate specifically

Key facts: α₂ββ'ω composition: β' binds DNA, β holds active site, α assembles enzyme + contacts UP element

Cis-regulatory DNA element at/near +1 start site where RNA pol + factors assemble. Prok: -10 (TATAAT), -35 (TTGACA), UP element (A/T rich, contacts α-CTD). Euk Pol II: TATA box (-25 to -30), Inr (overlaps +1), BRE, DPE, MTE.

Key facts: Promoter strength = frequency of transcription initiation. Strong promoter = consensus -10/-35 match. Only 10-20% of Pol II promoters have TATA box; CpG-island promoters lack TATA, use Inr/DPE instead

TATAAT consensus sequence ~10 bp upstream of transcription start in bacteria

Key facts: AT-rich → low melting temp → easy strand separation for open complex formation at +1

TTGACA consensus sequence ~35 bp upstream of transcription start; recognized by σ

Key facts: σ region 4.2 contacts -35; spacing between -35 and -10 = 17±1 bp (critical for alignment)

TATAA sequence ~25-30 bp upstream of eukaryotic Pol II transcription start; bound by TBP

Key facts: Bound by TBP (saddle shape, minor groove); bends DNA ~80°; positions +1 start site

Proteins (TFIID, TFIIB, TFIIF, TFIIE, TFIIH) required for Pol II to initiate transcription

Key facts: Ordered assembly: TFIID → TFIIB → TFIIF+PolII → TFIIE → TFIIH; forms preinitiation complex (PIC)

TFIID contains TBP (TATA-binding protein) + TAFs; first factor to bind the promoter

Key facts: TBP binds TATA box; TAFs (TBP-associated factors) recognize Inr, DPE, MTE core promoter elements

Dual-function GTF: (1) XPB subunit = 3'→5' helicase, unwinds ~12-14 bp at +1 for open complex. (2) Cdk7/cyclin H = kinase, phosphorylates CTD Ser5 → promoter escape + capping enzyme recruitment. Also functions in NER DNA repair (XPB/XPD mutations → xeroderma pigmentosum).

Key facts: 10 subunits total. XPB mutation → trichothiodystrophy (TTD) or Cockayne syndrome. α-amanitin does NOT inhibit TFIIH; it inhibits Pol II directly

Repeated heptad (Tyr-Ser-Pro-Thr-Ser-Pro-Ser) on Pol II largest subunit; 52 repeats in humans

Key facts: 52 heptad repeats (humans); Ser5-P by TFIIH → capping enzyme recruitment; Ser2-P by P-TEFb (Cdk9/cyclin T) → elongation/splicing/poly-A factors

Large multi-subunit complex bridging gene-specific transcription factors and Pol II

Key facts: ~30 subunits; head module contacts Pol II CTD, tail module contacts gene-specific activators; required for regulated transcription

Transcribes 45S pre-rRNA (yields 28S, 18S, 5.8S rRNAs) in the nucleolus

Key facts: Transcribes ~400 tandem rDNA repeats in nucleolus; produces >80% of total cellular RNA by mass

Transcribes tRNA, 5S rRNA, and some snRNAs

Key facts: Internal promoter (type 1/2) for tRNA/5S rRNA; upstream promoter (type 3) for U6 snRNA

Modified guanosine added to the 5' end of pre-mRNA co-transcriptionally

Key facts: Added co-transcriptionally after ~20-30 nt; 5'-5' triphosphate linkage; bound by CBC (nuclear) then eIF4E (translation)

~200 adenines added to 3' end of mRNA by poly-A polymerase (PAP) — template-independent. Functions: (1) stabilizes mRNA vs 3'→5' exonucleases, (2) aids nuclear export, (3) enhances translation (PABP-eIF4G interaction)

Key facts: CPSF binds AAUAAA → CstF binds GU-rich element → cleavage → PAP adds ~200 A's; PABP coats tail → stabilizes + aids export

Non-coding intervening sequence removed from pre-mRNA by splicing

Key facts: Average human gene: ~8 introns; some span >100 kb; begin GU, end AG (GT-AG rule in DNA); removed by spliceosome

Coding sequence retained in mature mRNA after splicing

Key facts: Joined after intron removal; can be coding, 5' UTR, or 3' UTR; exon shuffling drives protein domain evolution

5 snRNPs (U1, U2, U4, U5, U6) + ~200 proteins = megadalton complex. Catalytic core = U2+U6 snRNAs (ribozyme, no protein catalysis). Two transesterification reactions: (1) 2'-OH of branch-point A attacks 5' splice site → lariat, (2) free 3'-OH of exon 1 attacks 3' splice site → exons ligated, lariat released + debranched + degraded

Key facts: 5 snRNPs + ~200 proteins; catalytic core = U2/U6 snRNAs (ribozyme); two transesterifications → lariat + ligated exons

Small nuclear ribonucleoprotein particles (U1-U6) that form the spliceosome

Key facts: U1 base-pairs with 5' splice site; U2 base-pairs with branch point (bulges A); U6 replaces U1 and catalyzes reaction

Self-splicing intron using an external guanosine as nucleophile; found in rRNA of Tetrahymena

Key facts: External G cofactor attacks 5' splice site; 3'-OH of upstream exon attacks 3' splice site; found in Tetrahymena rRNA (Cech, 1982)

Self-splicing intron using an internal adenosine 2'-OH; produces a lariat

Key facts: Internal branch-point A (2'-OH) attacks 5' splice site → lariat; same chemistry as spliceosome; supports RNA world hypothesis

One gene → multiple mRNA variants by differential exon inclusion/exclusion. Types: exon skipping (most common), alt 5'/3' splice site, intron retention, mutually exclusive exons. >95% of human multi-exon genes undergo alt splicing

Key facts: SR proteins (Ser/Arg-rich) bind ESEs (exonic splicing enhancers) → promote exon inclusion. hnRNPs bind ESSs (exonic splicing silencers) → promote exon exclusion/skipping. Classic example: Drosophila Dsx (sex determination)

Small nucleolar ribonucleoprotein particles that guide rRNA modification (methylation, pseudouridine)

Key facts: Box C/D snoRNPs guide 2'-O-methylation; Box H/ACA snoRNPs guide pseudouridylation; ~200 modifications per rRNA

Ribozyme that cleaves the 5' leader of pre-tRNA

Key facts: RNA subunit = catalytic component; cleaves 5' leader of pre-tRNA; shared Nobel Prize with Cech (1989)

AAUAAA sequence in pre-mRNA that signals cleavage and poly-A addition ~20 nt downstream

Key facts: CPSF recognizes AAUAAA; CstF binds downstream GU-rich element; cleavage occurs ~10-30 nt after AAUAAA

Prok gene cluster: promoter-operator-structural genes, transcribed as single polycistronic mRNA. Lac operon = lacZ (β-galactosidase), lacY (permease), lacA (transacetylase). Dual control: negative (LacI repressor) + positive (CAP-cAMP)

Key facts: Allows coordinate regulation of metabolic pathways

Tetramer encoded by lacI gene (constitutively expressed). Binds operator (21-bp palindrome overlapping +1) → physically blocks RNA pol. Allolactose (lactose isomer) = inducer → binds LacI → allosteric conformational change → LacI releases operator → transcription proceeds

Key facts: Classic model of negative regulation; allolactose binding releases it

Cis-regulatory DNA element overlapping/adjacent to promoter. Lac: 21-bp palindrome at +1, repressor binds via helix-turn-helix motif. trp operon: operator + attenuator (leader peptide senses Trp-tRNA levels)

Key facts: The molecular OFF switch in negative control

Positive regulator (homodimer, helix-turn-helix). Low glucose → adenylyl cyclase active → cAMP rises → cAMP binds CAP → CAP-cAMP binds DNA upstream of promoter (-61) → bends DNA ~90° → enhances RNA pol α-CTD contact → 50-fold activation

Key facts: Classic model of positive control; links carbon source availability to gene expression

Cis-regulatory element containing clustered TF binding sites. Works at any distance (up to 1 Mb), any orientation (upstream/downstream/within introns). Contacts promoter via DNA looping (cohesin + CTCF define loop boundaries). Active enhancers marked by H3K27ac + H3K4me1

Key facts: Contains binding sites for multiple TFs; can work in any orientation and distance

Sequence-specific TF with modular structure: DNA-binding domain (DBD) + activation domain (AD). DBD types: helix-turn-helix, zinc finger (Cys₂His₂, 1 Zn²⁺ per finger), leucine zipper (coiled-coil dimerization), helix-loop-helix (HLH, homo/heterodimers). AD recruits Mediator/HATs/remodelers

Key facts: DBD types: helix-turn-helix, zinc finger (Cys₂His₂, 1 Zn²⁺ per finger), leucine zipper (coiled-coil dimerization + basic region), HLH (helix-loop-helix, homo/heterodimers). Methods: EMSA/gel shift (detects TF-DNA binding in vitro), DNase footprinting (identifies exact binding site on DNA), ChIP-seq (maps TF binding genome-wide in vivo), reporter gene assays (luciferase/GFP downstream of promoter/enhancer)

Negative TF that silences genes. Mechanisms: (1) recruit HDACs → deacetylate histones → compact chromatin, (2) recruit HMTs (e.g., SUV39H1 → H3K9me3, EZH2/PRC2 → H3K27me3), (3) compete with activator for same DNA site, (4) mask activator's AD (quenching). Example: Rb recruits HDAC to E2F-target promoters

Key facts: Polycomb group (PcG) = major eukaryotic repressors. PRC2 (EZH2 catalytic subunit) = writer (trimethylates H3K27 → H3K27me3). PRC1 = reader (chromodomain binds H3K27me3) + E3 ligase (ubiquitylates H2AK119). Trithorax group (TrxG) = antagonizes Polycomb, maintains active state. Rb recruits HDAC to E2F-target promoters → blocks cell cycle entry

~30-subunit complex with 4 modules: head (contacts Pol II CTD), middle (scaffold), tail (contacts gene-specific activators/enhancers), kinase module (CDK8, dissociable, can repress). Essential for converting activator signals into Pol II recruitment

Key facts: Required for ~90% of Pol II genes. CDK8 kinase module (dissociable 4th module) can phosphorylate TFs → positive or negative regulation. Head module contacts Pol II CTD, tail contacts activators. Mediator mutations → developmental disorders (MED12 mutations → FG/Opitz-Kaveggia syndrome, intellectual disability)

Physical bending of DNA that allows distant enhancer-bound TFs to contact promoter-bound factors

Key facts: Explains how enhancers 1000 kb away regulate their target genes

Ring-shaped protein complex that stabilizes DNA loops between enhancers and promoters

Key facts: SMC1/SMC3 heterodimer + RAD21 (kleisin) + SA subunit form ring that topologically embraces DNA. Loop extrusion: cohesin slides along DNA creating loops until blocked by convergent CTCF sites. Cohesin mutations → Cornelia de Lange syndrome (cohesinopathy). Also mediates enhancer-promoter contacts

Architectural protein that defines boundaries of chromosomal loop domains (with cohesin)

Key facts: 11 zinc fingers → recognizes ~20 bp consensus motif. Binds DNA in orientation-dependent manner (convergent CTCF sites block cohesin). Insulator function: prevents enhancer from activating wrong gene across TAD boundary. CTCF binding is methylation-sensitive (CpG methylation blocks CTCF → boundary lost → ectopic enhancer activation → disease, e.g., IDH-mutant gliomas)

HATs (p300/CBP, GCN5, PCAF) transfer acetyl group from acetyl-CoA to ε-amino group of lysine on H3/H4 tails. Key residues: H3K9ac, H3K14ac, H3K27ac (enhancer mark), H4K16ac. Neutralizes Lys + charge → weakens histone-DNA electrostatic grip → open chromatin (euchromatin)

Key facts: Bromodomain proteins (BRD4) = acetyl-lysine readers → recruit P-TEFb for transcription elongation. p300/CBP mutations → Rubinstein-Taybi syndrome. HDAC inhibitors (vorinostat, romidepsin) = FDA-approved cancer drugs (cause hyperacetylation → reactivate tumor suppressors). Acetyl-CoA = acetyl donor

Removal of acetyl groups from histones by histone deacetylases

Key facts: Restores positive charge → tightens chromatin → gene SILENCING

ATP-dependent machines (e.g., SWI/SNF) that slide, eject, or restructure nucleosomes

Key facts: Required to expose promoters/enhancers buried in nucleosomes

Decondensed, DNase I-sensitive chromatin. Marks: H3K4me3 (active promoter), H3K27ac (active enhancer), H3K36me3 (active gene body), hyperacetylated H3/H4. Replicates early in S phase. Contains ~92% of genes

Key facts: 10-nm fiber (beads-on-a-string) configuration. DNase I hypersensitive sites mark regulatory elements. Replicates early S phase. Accessible to TFs, RNA pol, remodelers. Contains ~92% of protein-coding genes

Condensed, DNase I-resistant, transcriptionally silent. 2 types: (1) Constitutive = permanent (centromeres, telomeres, satellite DNA), marked by H3K9me3 → HP1 binding. (2) Facultative = reversible (inactive X, imprinted genes), marked by H3K27me3 → Polycomb repressive complex (PRC2)

Key facts: Constitutive: centromeres (α-satellite DNA), telomeres, pericentromeric regions — marked by H3K9me3, bound by HP1 (chromodomain). Facultative: inactive X (Barr body, coated by Xist lncRNA), imprinted loci, Polycomb-silenced genes — marked by H3K27me3. Replicates late S phase. Position effect variegation: gene near heterochromatin boundary → stochastic silencing

DNMT3a/DNMT3b = de novo methyltransferases (establish new patterns). DNMT1 = maintenance methyltransferase (copies pattern to daughter strand after replication, recognizes hemimethylated CpG via UHRF1). Methyl group added to C5 of cytosine → 5-methylcytosine (5mC)

Key facts: Promoter CpG methylation → recruits MeCP2 + NCoR/HDAC complex → chromatin compaction → silencing. Gene body methylation correlates with active transcription. TET enzymes (TET1/2/3) = erasers: oxidize 5mC → 5hmC → 5fC → 5caC → base excision repair → unmodified C. 5-azacytidine/decitabine = DNMT inhibitors (cancer drugs, reactivate silenced tumor suppressors)

Region of DNA with high frequency of CG dinucleotides; often found at gene promoters

Key facts: When unmethylated → gene active; when methylated → gene silenced

Heritable changes in gene expression NOT due to changes in DNA sequence (e.g., methylation, histone marks)

Key facts: Explains how identical DNA in all cells produces different cell types

Silencing of one X chromosome in female mammals via Xist lncRNA and heterochromatin formation

Key facts: Xist lncRNA (~17 kb) coats inactive X in cis → recruits PRC2 (H3K27me3) + DNMT3b (DNA methylation) → heterochromatin (Barr body). Tsix = antisense lncRNA, blocks Xist on active X. Random in somatic cells (chosen ~day 5.5 in mouse). ~15% of genes escape inactivation. XCI = dosage compensation in XX mammals

Parent-of-origin gene expression: one allele silenced by DNA methylation established in germline. ~100 imprinted genes in humans. IGF2 = paternally expressed (maternal allele silenced). H19 = maternally expressed (paternal allele silenced)

Key facts: ~100 imprinted genes in humans. Prader-Willi = loss of paternal 15q11-13 (obesity, intellectual disability). Angelman = loss of maternal UBE3A at same locus (seizures, ataxia). Beckwith-Wiedemann = IGF2 overexpression (overgrowth). Imprint marks erased in primordial germ cells, re-established based on sex of new parent during gametogenesis. ICRs (imprinting control regions) regulate via CTCF-dependent insulators

~22 nt non-coding RNA that binds 3' UTR of target mRNA → translational repression + mRNA degradation

Key facts: Seed region (nt 2-8 of guide strand) base-pairs with 3' UTR of target mRNA (imperfect match = miRNA; perfect match = siRNA-like cleavage by Ago2). 1 miRNA can target ~hundreds of mRNAs. Mechanism: blocks ribosome scanning + recruits deadenylase (CCR4-NOT) → mRNA decapping → degradation in P-bodies. ~60% of human genes are miRNA targets. Fire & Mello 2006 Nobel (RNAi in C. elegans)

~22 nt double-stranded RNA that targets perfectly complementary mRNA for cleavage by RISC/Argonaute

Key facts: Used experimentally for gene knockdown (RNAi); also endogenous defense

Effector complex for RNAi. Core = Argonaute (Ago2 in humans has Slicer/endonuclease activity). Guide strand (antisense) loaded; passenger strand degraded. miRNA-RISC: imperfect match → translational repression. siRNA-RISC: perfect match → Ago2 cleaves mRNA between nt 10-11 of guide

Key facts: Ago2 = only human Argonaute with Slicer (endonuclease) activity. Slicer cleaves target mRNA between nt 10-11 of guide strand (requires perfect complementarity). RISC is catalytic — each complex degrades multiple mRNA molecules. siRNA-RISC: perfect match → cleavage. miRNA-RISC: imperfect match → translational repression + deadenylation

Combinatorial modifications on histone tails (acetylation, methylation, phosphorylation, ubiquitylation) form a code read by effector proteins. Writers: HATs, HMTs, kinases. Erasers: HDACs, HDMs (e.g., LSD1, JMJD), phosphatases. Readers: bromodomains (acetyl), chromodomains (methyl), PHD fingers

Key facts: Active marks: H3K4me3 (promoter), H3K36me3 (gene body), H3K27ac (enhancer). Silencing marks: H3K9me3 (HP1 → constitutive heterochromatin), H3K27me3 (Polycomb → facultative). Bivalent domains = H3K4me3 + H3K27me3 at same promoter in stem cells (poised genes). Writers: HATs, HMTs (SET domain). Readers: bromodomains (Ac-Lys), chromodomains (Me-Lys), PHD fingers. Erasers: HDACs, KDMs (LSD1, JmjC family)

3-nt mRNA unit read 5'→3' during translation. 64 codons: 61 sense (amino acids) + 3 stop (UAA/ochre, UAG/amber, UGA/opal). AUG = start (Met). Code is degenerate (redundant) but unambiguous. Wobble: position 3 of codon tolerates non-Watson-Crick pairing (inosine in tRNA anticodon pairs with U, C, or A)

Key facts: The basic unit of the genetic code; 64 codons total (61 amino acid + 3 stop)

Three-nucleotide sequence on tRNA that base-pairs with complementary mRNA codon

Key facts: The adaptor function of tRNA — matches amino acid to mRNA instruction

20 enzymes (1 per amino acid), each recognizes specific amino acid + all its cognate tRNAs. 2-step reaction: (1) aa + ATP → aminoacyl-AMP + PPi (activation), (2) aminoacyl-AMP + tRNA → aminoacyl-tRNA + AMP (transfer to 3'-OH of tRNA acceptor stem CCA). Class I: acylate 2'-OH. Class II: acylate 3'-OH

Key facts: Proofreading: editing site hydrolyzes mischarged aa-tRNA (e.g., IleRS editing site rejects Val). Error rate <10⁻⁴. PPi → 2Pi (pyrophosphatase) drives reaction forward. Net cost: 2 high-energy bonds per aa. tRNA identity elements: acceptor stem + anticodon. Class I synthetases acylate 2′-OH, Class II acylate 3′-OH

Prok 70S = 30S (16S rRNA + 21 proteins) + 50S (23S + 5S rRNA + 31 proteins). Euk 80S = 40S (18S rRNA + ~33 proteins) + 60S (28S + 5.8S + 5S rRNA + ~49 proteins). 3 tRNA sites: A (aminoacyl, incoming), P (peptidyl, growing chain), E (exit, deacylated). Peptidyl transferase = 23S/28S rRNA (ribozyme)

Key facts: Antibiotics target prok 70S: chloramphenicol (blocks peptidyl transferase, 50S), tetracycline (blocks A-site tRNA binding, 30S), erythromycin (blocks exit tunnel, 50S), streptomycin (causes misreading, 30S). Cycloheximide targets euk 80S (blocks translocation). Puromycin = aa-tRNA mimic, causes premature termination (both prok + euk)

Ribosomal site where incoming aminoacyl-tRNA binds, paired with the mRNA codon

Key facts: Entry point for new amino acids; accuracy checked here by decoding center

Ribosomal site holding the tRNA attached to the growing polypeptide chain

Key facts: The 'working bench' where the peptide bond was just formed

Ribosomal site where deacylated (empty) tRNA exits the ribosome

Key facts: Releases spent tRNA back to cytosol for recharging

Prok initiation: AGGAGG consensus, 5-10 nt upstream of AUG. Base-pairs with 3' end of 16S rRNA (anti-Shine-Dalgarno: 3'-AUUCCUCCACUAG-5'). Allows internal initiation → polycistronic mRNAs translated. Absent in eukaryotes (euk use 5' cap scanning)

Key facts: Allows internal initiation on polycistronic mRNAs; absent in eukaryotes

Cap-binding protein in eIF4F complex (eIF4E + eIF4G scaffold + eIF4A helicase). eIF4E binds m7G cap → eIF4G bridges to PABP (circularizes mRNA) + recruits 43S PIC. Rate-limiting for translation initiation

Key facts: 4E-BP sequesters eIF4E when hypophosphorylated → blocks cap-dependent translation. mTOR phosphorylates 4E-BP → releases eIF4E → translation ON. eIF2 regulation: eIF2-GTP delivers Met-tRNAᵢ to 40S; eIF2α phosphorylation (by kinases: HRI=heme, GCN2=amino acids, PERK=ER stress, PKR=dsRNA/viral) → global translation inhibition + selective ATF4 translation. IRE/IRP system: iron low → IRP binds IRE in ferritin mRNA 5'UTR → blocks translation; IRP binds TfR mRNA 3'UTR → stabilizes it

Multiple ribosomes simultaneously translating a single mRNA molecule

Key facts: Allows efficient protein production from one mRNA

Catalytic activity (in large ribosomal subunit rRNA) that forms peptide bonds

Key facts: Ribozyme — rRNA catalyzes the reaction, not protein

Prok: RF1 recognizes UAA + UAG, RF2 recognizes UAA + UGA (GGQ motif mimics tRNA, triggers hydrolysis of peptidyl-tRNA ester bond), RF3 = GTPase recycles RF1/RF2. Euk: eRF1 recognizes all 3 stops (single factor), eRF3 = GTPase. After release: ribosome recycling factor (RRF) + EF-G split 70S → 30S + 50S

Key facts: RF1/RF2 GGQ motif enters peptidyl transferase center, triggers ester bond hydrolysis. Suppressor tRNAs can read through stop codons. Selenocysteine = 21st aa, encoded by UGA + SECIS element in 3'UTR. Puromycin = structural mimic of aminoacyl-tRNA (Tyr), enters A site, forms peptide bond, causes premature termination (used experimentally, targets both prok + euk)

Proteins (Hsp70, Hsp60/GroEL) that assist proper protein folding without being part of the final structure

Key facts: Prevent aggregation; provide a protected environment for folding

Chaperone (DnaK in bacteria). ATP-bound = open lid, low substrate affinity → binds hydrophobic patches. ATP hydrolysis (stimulated by Hsp40/DnaJ co-chaperone) → closed lid, tight grip on substrate. Nucleotide exchange factor (GrpE/BAG1) replaces ADP → substrate released → refolds or transferred to chaperonin

Key facts: Acts co-translationally (ribosome-associated Hsp70/RAC) + post-translationally + during heat shock (HSF1 induces Hsp70 expression). Required for mito/chloro import: matrix Hsp70 (mtHsp70) pulls unfolded polypeptide through TIM23 channel (Brownian ratchet model). DnaK/DnaJ/GrpE = bacterial Hsp70 system

GroEL = 2 stacked 7-mer rings (14 subunits total, each ~57 kDa). GroES = 7-mer co-chaperonin lid. Substrate (~20-60 kDa) binds hydrophobic interior of open ring → GroES caps → 7 ATP bind → conformational change makes cavity hydrophilic → substrate folds inside for ~10 sec → ATP hydrolysis → GroES + substrate released

Key facts: 7 ATP consumed per folding cycle (per ring). Only ~10% of E. coli proteins require GroEL (mostly 20-60 kDa). Euk equivalent = TRiC/CCT (8-subunit ring, no detachable lid). Anfinsen cage model: hydrophilic cavity prevents aggregation, allows single-molecule folding

76-aa protein (8.5 kDa), highly conserved. Conjugated to substrate Lys via isopeptide bond (C-terminal Gly). Pathway: E1 (ubiquitin-activating, 2 in humans, uses ATP) → E2 (conjugating, ~40 types) → E3 (ligase, ~600+ types, provides substrate specificity) → polyUb chain

Key facts: K48-linked polyUb (≥4 Ub) = proteasomal degradation. K63-linked = signaling (NF-κB, DNA repair). Mono-Ub = endocytic sorting, histone regulation (H2BK120ub). 26S proteasome = 20S core (4 stacked 7-mer rings: α7β7β7α7; β1/β2/β5 = proteolytic active sites) + 19S regulatory particle (recognizes polyUb, has ATPases to unfold + feed substrate through α-ring gate). DUBs (deubiquitinases) recycle Ub before substrate enters 20S

Large barrel-shaped protease complex that degrades ubiquitylated proteins to peptides

Key facts: Regulated protein destruction; requires ATP; recycles ubiquitin

Ubiquitin-activating (E1), conjugating (E2), and ligase (E3) enzymes in the ubiquitin pathway

Key facts: E3 provides substrate specificity — determines WHICH proteins get ubiquitylated

Process where cells degrade their own organelles/proteins by enclosing them in autophagosomes that fuse with lysosomes

Key facts: Bulk degradation for recycling during starvation or for quality control

System where protein half-life is determined by its N-terminal amino acid (N-end rule)

Key facts: Destabilizing N-terminal residues target proteins for rapid ubiquitylation

N-terminal ~16-30 aa: positively charged n-region + hydrophobic h-region (core, 7-15 hydrophobic aa) + polar c-region (signal peptidase cleavage site). Recognized co-translationally by SRP (signal recognition particle) when it emerges from ribosome exit tunnel

Key facts: SRP = 6 proteins + 7SL RNA (in mammals). SRP binds signal peptide emerging from ribosome exit tunnel → pauses translation → docks at SRP receptor (SRα/SRβ, GTPases) on ER membrane → ribosome-nascent chain transferred to Sec61 translocon → translation resumes co-translationally → signal peptidase cleaves signal in ER lumen. Type II membrane proteins use signal-anchor (NOT cleaved)

Covalent changes to proteins after synthesis: phosphorylation, glycosylation, acetylation, etc.

Key facts: Regulate protein activity, localization, interactions, and stability

Enzyme that transfers phosphate from ATP to serine/threonine/tyrosine residues on proteins

Key facts: Master regulators of cell signaling; ~500 kinases in human genome

Enzyme that removes phosphate groups from proteins, reversing kinase action

Key facts: Works opposite to kinases; together they create reversible signaling switches

3rd codon position tolerates non-Watson-Crick pairing at anticodon position 1: G-U pairs allowed; inosine (I) in anticodon pairs with U, C, or A → one tRNA reads up to 3 codons. Minimum 31 tRNAs needed (not 61) to decode all sense codons.

Key facts: Explains why only ~45 tRNAs can read all 61 sense codons; inosine (I) in anticodon pairs with U, C, or A

~16-30 aa N-terminal peptide: positively charged n-region → hydrophobic h-region (7-15 Leu/Ala, forms α-helix in Sec61 channel) → polar c-region with signal peptidase cleavage site (Ala-X-Ala rule)

Key facts: Recognized co-translationally by SRP54 methionine-rich M domain; inserts into Sec61 translocon lateral gate; cleaved by signal peptidase on ER lumenal side

Ribonucleoprotein (6 proteins + SRP RNA) that binds signal sequence and pauses translation

Key facts: Molecular escort: bridges ribosome to ER membrane

ER membrane protein that binds SRP-ribosome complex; triggers GTP hydrolysis to release SRP

Key facts: Docking station on the ER for incoming ribosomes

Protein channel (3 subunits: α,β,γ) in ER membrane through which polypeptides are threaded

Key facts: Has a plug that opens when signal sequence inserts; lateral gate for transmembrane domains

ER lumenal enzyme that cleaves the signal sequence from translocating proteins

Key facts: Removes the 'address label' once delivery is confirmed

Hydrophobic transmembrane domain that halts translocation and anchors protein in ER membrane

Key facts: Determines single-pass membrane protein topology

ER-resident chaperone that assists protein folding in the ER lumen

Key facts: Binds unfolded proteins as they enter; also sensor for UPR

Addition of 14-sugar oligosaccharide to asparagine (Asn-X-Ser/Thr) in ER from dolichol carrier

Key facts: Aids folding, prevents aggregation, provides quality control signals

Addition of sugars to serine/threonine hydroxyl groups; occurs in the Golgi

Key facts: Further modification for cell surface and secreted proteins

Coat protein complex II; mediates anterograde transport (ER → Golgi)

Key facts: Selective: concentrates cargo proteins with ER exit signals

Coat protein complex I; mediates retrograde transport (Golgi → ER)

Key facts: Retrieves escaped ER-resident proteins (recognize KDEL signal)

Vesicles coated with clathrin triskelion; mediate transport from Golgi/plasma membrane

Key facts: Used in receptor-mediated endocytosis and M6P lysosomal sorting

Lys-Asp-Glu-Leu C-terminal sequence that marks ER-resident soluble proteins for retrieval from Golgi

Key facts: KDEL receptor in Golgi captures escaped proteins and returns them via COPI

Phosphorylated mannose residue added to lysosomal enzymes in cis-Golgi; recognized by M6P receptor

Key facts: The 'lysosome address tag'; recognized by M6P receptor in trans-Golgi for sorting

v-SNAREs (on vesicle) and t-SNAREs (on target) that mediate membrane fusion via coiled-coil zippering

Key facts: Ensure vesicles fuse with correct target membrane; specificity mechanism

Small GTPases on vesicle surfaces that regulate vesicle targeting and tethering

Key facts: Act as molecular switches: GTP-bound = active, GDP-bound = inactive

Quality control: misfolded ER proteins retrotranslocated to cytosol and degraded by proteasome

Key facts: Prevents accumulation of defective proteins in the secretory pathway

Signaling pathway activated when misfolded proteins accumulate in ER; upregulates chaperones

Key facts: Adaptive response: increases ER folding capacity; if overwhelmed → apoptosis

Default pathway: continuous vesicle fusion with plasma membrane without specific signal

Key facts: How most membrane proteins and ECM components reach the surface

Signal-triggered release of stored secretory vesicles (e.g., neurotransmitters, hormones)

Key facts: Requires external stimulus (Ca²⁺, hormone); contents stored in dense-core granules

Glycosylphosphatidylinositol lipid anchor attached to C-terminus; tethers protein to outer membrane leaflet

Key facts: Alternative to transmembrane domain; assembled in ER, added to protein post-translationally

ER enzyme that catalyzes formation and rearrangement of disulfide bonds

Key facts: Oxidizing ER environment (unlike reducing cytosol) enables S-S bond formation

Double-membrane organelle; site of oxidative phosphorylation and ATP production

Key facts: The cell's power plant; contains own genome; evolved from α-proteobacteria

Folds of the mitochondrial inner membrane that increase surface area for oxidative phosphorylation

Key facts: More cristae = more ETC complexes = more ATP production capacity

Inner compartment containing citric acid cycle enzymes, mtDNA, ribosomes

Key facts: The working interior of mitochondria where pyruvate and fatty acids are oxidized

Space between inner and outer mitochondrial membranes; similar composition to cytosol

Key facts: Where protons accumulate during electron transport → pH lower than matrix

Channel proteins in mitochondrial outer membrane allowing free diffusion of molecules <1000 Da

Key facts: Makes outer membrane freely permeable to small molecules (unlike inner membrane)

Series of protein complexes (I-IV) in inner membrane that transfer electrons from NADH/FADH₂ to O₂

Key facts: Couples electron transfer to proton pumping across inner membrane

Mitchell's theory: proton gradient across inner membrane drives ATP synthesis by ATP synthase

Key facts: Electrochemical gradient (ΔΨ + ΔpH) = proton-motive force

Rotary enzyme in inner membrane that synthesizes ATP from ADP + Pi using proton flow

Key facts: F₀ portion = proton channel in membrane; F₁ = catalytic head in matrix

Combined electrochemical potential (voltage + pH gradient) across inner mitochondrial membrane

Key facts: Drives both ATP synthesis and metabolite transport

N-terminal targeting signal (15-55 aa, positively charged amphipathic helix) for mitochondrial import

Key facts: Removed by matrix processing peptidase (MPP) after import

Translocase of the Outer Membrane; general entry point for all mitochondrial protein import

Key facts: Receptor subunits recognize presequences and internal signals

Translocase of the Inner Membrane; imports presequence-containing proteins to matrix or inner membrane

Key facts: Driven by membrane potential (negative inside attracts positive presequence)

Second inner membrane translocase; inserts multi-pass carrier proteins with internal signals

Key facts: Uses Tim9-Tim10 chaperones in IMS for delivery

Small chaperones in intermembrane space that escort hydrophobic proteins between TOM and TIM22

Key facts: Prevent aggregation of hydrophobic inner membrane proteins in aqueous IMS

Protease in mitochondrial matrix that cleaves the presequence after protein import

Key facts: Removes the 'address label' once the protein reaches its destination

Sorting and Assembly Machinery in outer membrane; inserts β-barrel proteins

Key facts: After proteins pass through TOM, SAM inserts them into the outer membrane

Double-membrane + thylakoid membrane organelle; site of photosynthesis in plants

Key facts: Three membranes → three compartments (IMS, stroma, thylakoid lumen)

Internal membrane system of chloroplasts; contains photosystems and ATP synthase for light reactions

Key facts: Where light energy is captured and converted to chemical energy

Aqueous interior of chloroplast (outside thylakoids); contains Calvin cycle enzymes and chloroplast DNA

Key facts: Equivalent to mitochondrial matrix; site of carbon fixation

Translocase of Outer/Inner Chloroplast membrane; imports nuclear-encoded chloroplast proteins

Key facts: Transit peptides (not presequences) target proteins; require GTP + ATP

N-terminal targeting signal for chloroplast import; cleaved by stromal processing peptidase

Key facts: Differs from mito presequence: not positively charged amphipathic helix

Mitochondria evolved from α-proteobacteria; chloroplasts from cyanobacteria engulfed by ancestral eukaryote

Key facts: Supported by: own DNA, double membrane, bacterial-like ribosomes, binary fission

Single-membrane organelle containing oxidative enzymes (catalase, oxidases); involved in fatty acid β-oxidation

Key facts: Generates H₂O₂ as byproduct; catalase converts it to H₂O + O₂

Genes encoding peroxin proteins required for peroxisome biogenesis and protein import

Key facts: Mutations cause Zellweger syndrome (peroxisome biogenesis disorder)

C-terminal tripeptide (SKL or conservative variant) that targets most matrix proteins to peroxisomes

Key facts: Recognized by Pex5 receptor in cytosol; most common peroxisomal import signal

N-terminal nonapeptide signal targeting a few peroxisomal matrix proteins; recognized by Pex7 receptor

Key facts: Only used by a few proteins (e.g., thiolase); cleaved after import in some organisms