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Bi4025en
Molecular Biology
Mgr. Jiří Kohoutek, Ph.D.
1    Department of Experimental Biology
Lecture 6
• Posttranslational processing of proteins.
2    Department of Experimental Biology
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Generation of maturated functuional protein
Newly svnthetized propeptide chain
Folding.
o Noncovalent binding of cofactors.
Covalent modifications o Glycosylation, phosphorylation, acetylation, etc.
Assembly
o Noncovalent binding of other protein
subunits/partners. o Maturated functional protein.
3    Department of Experimental Biology
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Post-translation modifications are key to proteome diversity
• Genome comprises 20,000 to 25,000 genes.
• Changes at the transcriptional and mRNA levels increase the size of the transcriptome relative to the genome.
Myriad of different post-translational modifications exponentially increases the complexity of the proteome relative to both the transcriptome and genome .
The proteome is estimated to encompass over 1 million proteins.
-2(}-25r0D0 genes
AAA
Alternative promoters Alternative Splicing mRNA editing
Transcriptome -100,000 transcripts
Post-transfational modifications
Protecme si,000,000 proteins
SP
4    Department of Experimental Biology
https://www.thermofisher.com/cz/en/home/life-science/protein-biology/protein-biology-learning-center/protein-biology-resource-library/pierce-protein-methods/ove rview-post-translational-modification.html
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Interactions in an Organism Compose the Interactome
Proteome:
• Complete set of proteins produced by genetic material of an organism.
Interactome:
• Complete set of protein interactions in an organism.
: .....; ■
AN roArt W> J* 3" f. Vi * i <J i rtů n
1101)»» <™nwjoiC«timv
5    Department of Experimental Biology
https://slideplayer.com/slide/5746723/
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Protein synthesis in three levels of modifications
20 Amino acids + 20 tRNAs
Pre-translational Modifications
I
20 aa - tRNAs
Co-translational Modifications
I
Nascent polypeptide
Post-translational Modifications
I
Complete polypeptide
6    Department of Experimental Biology _ _ T
O U J.
Co-translational and Post-translational modifications
Post-translational modifications influence protein:
o Charge
o Conformation
o Size
Effects of post-translational modifications on protein:
o Stability
o Biochemical activity
o Protein targeting (localization)
o Protein signaling (protein-protein interaction)
Localization
Activity
[ Signal input ) Enzyme^
PTM crosstalk
w Enzyme , State 'w"5--©
[Signal output J
Conformation
— i
Binding
Turnover
7    Department of Experimental Biology
CELL, VOLUME 108, ISSUE 4, P557-572, FEBRUARY 22, 2002
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Protein synthesis in three levels of modifications
Levels
1. Pre-translational
2. Co-translational
3. Post-translational
8    Department of Experimental Biology
Modifications
a) Selenocysteine tRNA
b) Non-standard/natural amino acid tRNA
- dansylalanine (fluorescent reporter)
- phosphoserine, phosphothreonine, and phosphotyrosine (production of translational proteins in E coliwith Eukaryotic post-translational modifications )
a) Signal sequence celavage
b) N-Glycosylation
a) Phosphorylation
b) Acetylation
c) O-Glycosylation
d) Methylation
e) Lipidation
f) Proteolytic cleavage
g) Protein splicing
h) Ubiquitination, Sumoylation
https://slideplayer.com/slide/12777240/
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• Pre-translational modifications
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9    Department of Experimental Biology _ _ T
O 0 J.
Pre-translational modifications
Selenocysteine-tRNA is initially charged with serine. Then the attached serine is enzymatically modified to form selenocysteine.
HSe-
(Ser) + ATP
tRNAl5"')6"'
AMP+PP1
Ser.tRNAIs"|S«
10 Department of Experimental Biology
HN
0=S=0O
NH:
Adv Nutr. 2011 Mar; 2(2): 122-128. https://www.sigmaaldrich.com/CZ/en/product/sigma/d0125
H3C CH3
Alanine - conjugated to the fluorophore 5-(dimethylamino)naphthalene-l-sulfonyl is Dansyl-L-alanine. The unnatural amino acid is incorporated into the proteins by use of a mutated aminoacyl-tRNA synthetase specific for dansyl-L-alanine.
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• Co-translational modifications
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11   Department of Experimental Biology _ _ T
O 0 J.
N-terminal signal sequence
N-terminal signal sequences
• N-terminal signal sequence mediates targeting of nascent secretory and membrane proteins to the endoplasmic reticulum (ER) in a signal recognition particle (SRP)-dependent manner.
• Signal sequences have a tripartite structure, consisting of a h-region (hydrophobic core region) flanked by an n-region and c-region.
• The c-region contains the signal peptidase (SPase) consensus cleavage site. Usually, signal sequences are cleaved off co-translationally.
I_,
N —I    n    I     h     I c H
MKWVTFlSLLF5SAYS-|album i n WDSKG55QKGSRLLLLLWSNLLLCQGVVS-I prolactin-^ MGQ|\mAFEALPHIID£VINirWIIVLIIira
MPhH(^SPTGSSDaLSGKKQRPHLAiRRKRRRE^
12  Department of Experimental Biology http://www.signalpeptide.de/
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N-terminal signal sequence
Endoplasmic reticulum
ribosome with nascent protein
<2u
N
im
translocon SRP
receptor
■ + ^. I*     ► • •••••••••••
SPase C
signal sequences affect protein targeting, insertion and their cleavage in a qualitative and quantitative manner
signal peptide by SPP
membrane-inserted signal peptide
release of a signal peptide from the ER membrane
13 Department of Experimental Biology
http://www.signalpeptide.de/
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Protein glycosylation
Protein glycosylation
• One of the major post-translational modifications of many cell surface and secreted proteins.
• Significant effects on protein folding, conformation, distribution, stability and activity.
Selection of sugar ranges from simple monosaccharide to highly complex branched polysaccharide chains.
Dol-PP
• The sugar residues are often used as molecular flags or recognition signals to other cells that come in contact with them.
N-acety!glucosamine
5' mRNA
14 Department of Experimental Biology
https://www.thermofisher.com/cz/en/home/life-science/protein-biology/protein-biology-learning-center/protein-biology-resource-library/pierce-protein-methods/ove rview-post-translational-modification.html
Adv Neurobiol. 2014; 9: 47-70.
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Protein glycosylation
• Two types of glycosylation:
o N-linked - occurs on ASPARAGINE (N) residues within an X-N-X-S or X-N-X-T sequence - co-translational.
o O-linked occurs on the side chain hydroxyl oxygen of either SERINE (S) or THREONINE (T) residues determined not by surrounding sequence, but by secondary and tertiary structure- post-translational.
• N-linked glycosylation begins with a "tree" of 14 specific sugar residues that is then pruned and remodeled, but remains fairly large.
• O-linked glycosylation is based on sequential addition of individual sugars and does not usually extend beyond a few residues.
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Glycosyalation
Ribosome
Asparagine - Asn
• Glycosylation, both of which requires import of the target polypeptide into the ER first, but O-linked glycosylation is achieved in the Golgi apparatus.
16 Department of Experimental Biology
https://pubmed.ncbi.nlm.nih.gov/23094261/
T
R
l/VA P   Dotichol phosphate
NA<ulylg!j<Qv.imin.> (GI<NAc)
O    r.'ar-osc (Man) O Glucoi«(Glc)
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N-glycosylation
• N-glycosylation begins before a protein translation, as the dolichol diphosphate /pyrophosphate lipid, in the ER without being triggered by translation or protein entry.
• Lipid-glycan are bound Asp by the multisubunit oligosaccharyltransferase (OST).
• Glycosyltransferase catalyzes each step.
• Sugar substrates are sugar nucleotides, not isolated sugar molecules.
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N-glycosylation
ER lumen
Asn XSer.-Thr
o cr
I J J
Cytosol
^ - N-Acetylglucosamine # = Mannose O o'.:oic A = Galactose O Sacked
Transport to Golgi body
-lift l-I-l-f t t-t t * f:l-i l Í I:I H l *=t t «=t 11 l-i-t-i-Ull i-t t«t-l t-M-i i * t ti«I t-I-l t«:i I i-i i-t 1111111 i 11 <
Cc-:g !j~ic-
[>UDP UDP
and/or OCMP CMP
• The glucose residues are sequentially removed by two a-glucosidases (a-GIc l-ll) and an initial Man residue is removed by the ER a-mannosidase (ER a-Man).
• After a quality-control checkpoint, the glycoprotein moves to the Golgi apparatus for additional trimming by a-mannosidase I and II (a-Man l-ll) and further glycan modifications.
• A cis-to-trans distribution of glycosidases and transferases facilitates further processing by these carbohydrate-modifying enzymes to create a plethora of N-glycoforms that often terminate with sialic acid moieties.
Nature Reviews Nephrology, 2019, volume 15, pages 346-366. Wl U 111 I
18 Department of Experimental Biology https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N- O n T
linked_Protein_Glycosylation_Begins_in_the_ER O L» 1
• Post-translational modifications
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19 Department of Experimental Biology _ _ T
O 0 J.
Post-translational modifications - PTMs
phosphorylation
ubiquitiria'ron
P ost-tra n slational modifications
5UMOyla1;on
More than 300 PTMs are currently known.
Addition of chemical groups (e.g. phosphate or acetate).
Addition of complex molecules (e.g. carbohydrates or lipids).
The covalent linkage of small proteins (like ubiquitin, ubiquitin-like proteins (UBLs), sumo).
Cleavage and Splicing.
Modification of specific amino acids (like deamidation or eliminylation).
Department of Experimental Biology       Journal of Experimental Botany, Volume 69, Issue 19, 31 August 2018, Pages 4499-4503
vbiquifiu-iifte
proteolysis
deamidation eliniiiiylation
AMPytation
ADP-riiWSViS'iori
glycosyldtion
scylfltion pre relation
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Post-translational modification are carried out by enzymes
Phosphorylation (X = Ser, Tyr, Thr) / Eliminylation (X = Thr)
kinase phospholyase phosphate
x        ATP      ADP         £ Pi
^  ^ ^ f orotein^ ^m^^L
(protein) ^
' 7 s
P. H20 phosphatase
Acetylation (X = Lys, Sen Thr) acetyltransferase
Y      acetyl-coA coA
(protein) (protein)^,
acetate H20 deacetylase
acetate ■
X
^(protein)
AMPylation (X = Tyr, Thr)
AMPylator v ATP PP.
rproteinj ^
AMP H20 AMP hydrolase
AMP X
(protein)
Glucosylation (X = Thr, Ser)
glucosyltransferase g[ucose
UDP-glucose UDP
(protein)^
X i_
glucose glucosylhydrolase
^(protein)
H20
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21   Department of Experimental Biology FEBS Letters, Volume 584, Issue 13, 2 July 2010, Pages 2748-2758
O 0 J.
Post-translational modification are carried out by enzymes
ADP-ribosylation (X = Arg, Cys, Asn)
ADP-ribosyltransferase ADP.ribose
X
NAD
nicotinamide
^ protein^
ADP-ribose H20 ADP-ribosylhydrolase
^proteiňj
Deamidation / Polyamination
deamidase polyamine transferase
polyamine i
Gin
Ubiquitylation / UBL conjugation {X = Lys)
Ubi/UBL conjugation machinery Ubj/UBL Ubi/UBL + ATP AMP+PP,
X
JL
^protein^) ^
X
Ubi/UBL
"=š-
H20
Ubi/UBL protease
^ (protein^
Proteolysis
protease
^    NH     HO        „    polyamine   NH ■ Glu      * Gin 3 Gin
^protein^ (protein) -► (protein) (protein)
H20
tein
22 Department of Experimental Biology
FEBS Letters, Volume 584, Issue 13, 2 July 2010, Pages 2748-2758
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Post-translational modification are carried out by enzymes
0
o-s-o"
1
o
K n Tyrosine sulfation h\
0     Lysine acetyiahon
D
\
hn ,
HO,
5f*
Glycosylation
hn
Lysine ubtqui'jaaton
-n-^V 'UN'y' "^n^V Hq h   0 H q
Lysine methylabon
H^v^     HjAvnC -"nv^
HN hn hf'.
""TIT   ""«T    "K o
Arganne methyMton
23 Department of Experimental Biology
Phospho kinase Tyrosine phosphatase Ubiquitin ligase Deubiquitylase/deneddylase AMPylator
ADP-ribosyl transferase
Acetyltransferase
Deacetylases
Methyl transferase
Demethylase
Etc...
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Phosphorylation
Principally on SERINE, THREONINE or TYROSINE residues.
Also known as Phospho regulation.
Critical role in cell cycle, growth, apoptosis and signal transduction pathways.
O-phosphorylalion at serine residue .OH
H
24 Department of Experimental Biology
0
0=P-0* ATP       ADP ^0
\ / ,
H
Non-Phosphorated Protein
[ h
ATP
Ser-Thr Kinase ADP
Pi
Ser-Thr Phosphatase
-P
phosphorated Protein
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Phosphorylation affects protein capability
TRENDS tn Pharmacological Sciences
25  Department of Experimental Biology
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Phosphorylation
—
y.-rl70##Thfl76
Cycürt H) tCAK1
phtuphalase
9
t
Thi-161
TyilS ThTl&l
$0
Inactive pnp-kinase ftclivE* kinase (MPFF
O O
Npwfjr made cvclln B
IníiHvB Olui
O o
o o
00C
J
• As cyclin B is synthesized during S and G2 phases of the cell cycle, it associates with Cdc2.
• Active CDK-activating kinase (CAK) phosphorylates Cdc2 at threonine 161, stabilizing its association with cyclin B
• Wee1 and Myt1 phosphorylates inhibitory sites, threonine 14 and tyrosine 15.
• Final activation is triggered by dephosphorylation of Thr14 and Tyr15 by CDC25 phosphatase.
26 Department of Experimental Biology
Current Biology, Volume 5, Issue 1, January 1995, Pages 40-42
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Acetylation
Acetylation is one of the major post-translational protein modifications in the cell, with manifold effects on the protein and the metabolome level.
• Covalent attachment of an acetyl group eliminates the positive charge (+) of the amino group, thus affecting local electrostatic properties.
• These reactions are catalyzed by various N-terminal and LYSINE acetyltransferases.
• Involved in regulation of transcription factors, histones, effector proteins, molecular chaperons and cytoskeletal proteins.
27 Department of Experimental Biology
Experimental & Molecular Medicine, 2018, volume 50, pages1-13.
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Acetylation
• N-terminal acetvltransferases (NAT) transfer an acetyl group (CH3CO) to an a-amino group of protein N-termini.
• Acetvltransferases (KATs) catalyze the transfer of an acetyl group (CH3CO) to the £-amino group of LYSINE (K) side chains.
• NATs and KATs use acetyl-CoA (Ac-CoA) as a donor of acetyl group.
• In the case of lysine acetylation, the acetyl moiety may be removed by lysine deacetvltransferases (KDACs), making it a reversible protein modification - deacetylation.
N-terminus Na Acetyl N-terminus
(Nt) (AcNt)
28 Department of Experimental Biology
Experimental & Molecular Medicine, 2018, volume 50, pages1-13.
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N-terminal Acetylation
N-terminal acetylation (Nt-acetylation, AcNt) is a common protein modification, affecting an estimated 80% of all human protein species to a varying extent.
Nt-acetylation has many functions in the cell.
o Targets proteins for polyubiquitination and proteasomal degradation or protects against such degradation.
o Proper folding of some proteins.
o Protein-protein interactions.
o Targets some proteins for membranes.
b
Ai.
Protein half-life
At)
Folding.
Complex formation
Membrane targeting
29 Department of Experimental Biology
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Lysine Acetylation
Relaxed hromatjn
HDAC inhibitors (e>g-, wirinostjit, cntinostat)
Altered gene lion
Altered biological effects	in malignant tells
1 Proliferation	A Cell cycle
1 Migration	1 Cell death
• Histone acetylation and deacetvlation are essential parts of gene regulation.
• These reactions are typically catalyzed by enzymes with "histone acetvltransferase" (HAT) or "histone deacetvlase" (HDAC) activity.
• Acetylation of histones alters accessibility of chromatin and allows DNA binding proteins to interact with exposed sites to activate gene transcription and downstream cellular functions.
30 Department of Experimental Biology
https://www.wikiwand.com/en/Histone_acetylation_and_deacetylation
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Lysine Acetylation
Histories H2A, HS8, H4
Metabolic enzymes
GAPDH,
Enolase
Transcription GAT A lint finger, bHLH
Translation Initiation factor IF-3
Secondary metabolism Cytochrome P450 72 Al
Signal transduction Lectin-líke receptur kinase 1
RNA processing Exonuclease
Protein Stability £3 SUMO ligasÉ 51ZZ
Aranadtllo repeat Protein
Transposan & Retrotran&po&an Mutator & En/Spm sub-classes Ty3-gypsy Tyl-copta
31   Department of Experimental Biology
PLoS ONE 9(2): e89283. doi:10.1371/journal.pone.0089283
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Methylation
Addition of methyl group to a protein to
eliminate positive charge. Fr<"",5lno M"h"""""
LysorK Kmel Kmo2 Kmo3
Usually at LYSINE or ARGININE sc,™ m~% residues, also HISTIDINE.
Lysine contains a primary e-amine. spacefilling
J 1 J Structures
V R
MNh ©N-^t ©."-"Mt ©N
Methyl donor is S-adenosvlmethionine ^   ^     ^ jA
(SAM). Electrostatic .«> 9 i
Potential Surface
Enzyme for this is methyltransferase.
32  Department of Experimental Biology
Chem. Rev. 2018, 118, 14, 6656-6705
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Methylation
RNP granule ■ SMN
• FU5
•FMR1 / •CAPRIN1
• C3BP
Mitochondrion
• NDUFS2 •TDRKH
Focal adhesion •ACTN1
• EZR
• ITCA2
• DOCK7
Ribosome	Nuclear speckle	Nucleolus
• FMR1	•SRSF2	• FMR1
• RPS24	• RBM15	• PARP1
• LARP4B	• SF3B1	•CAR1
• EIF4G1	•PRPF3	• NOP56
Cytoskeleton • CAMKII
ACTN1
EZR
COBL
	
• RNA metabolic process	• Cellular response to DNA damage
• RNA processing	• Protein folding
• Chromosome organization	• Gene expression
• Aromatic, heterocycle and nucleic acid	• Viral process
metabolic process	• Microtubule-based process
• Co-translational protein targeting to membrane	• Ribosome
Protein, lysine and arginine, methylation function in:
• Epigenetic regulation.
• DNA damage response.
• Signaling pathways.
• Membrane less organelles by arginine methylation.
33 Department of Experimental Biology
Nature Reviews Drug Discovery volume 20, pages509-530 (2021)
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Methylation - Lysine
H H
\/ NH* I
(CH2)4
Lysine
H  (ch) (cH^^h)
NH*
I
(9H2)4
KMT
KDM
KMT
NH'
I
<CH2)4
Lys
KDM
Lys
Mono-methyl lysine
Di-methyl lysine
KDM
34 Department of Experimental Biology
(CH2)4
KMT
KDM
Lys
Tri-methyl lysine
Recruitment/ regulation
Lysine can be methylated like mono-, di- or trimethylated (Kme1, 2 or 3) through the addition of a methyl group to its terminal side-chain 8-amine.
Lysine methylation dynamics are controlled by the regulated action of KMTs to add and KDMs to remove the methyl.
Once the methyl modification has been made to the lysine, it can result in either the recruitment of binding proteins or direct effects to regulate protein function.
FEBS Journal, 2017, Vol. 284, 2732-2744.
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Methylation - Lysine
Methylation of K310 leads to translational repression of NF-kB through the recruitment of the EHMT1 (Euchromatic Histone Lysine Methyltransferase 1).
Recruitment of EHMT1 increases the localized methylation of H3(K9me2), resulting in the transcriptional repression of NF-kB target genes.
Serine phosphorylation of S311 blocks the binding of EHMT1 to K310, relieving the methylation-induced translational repression.
@3
SETD6 / \ Protein Kinase C
MBD recruitment
—I     Target genes
I Transcriptional repression
Active transcription
35 Department of Experimental Biology
FEBS Journal, 2017, Vol. 284, 2732-2744.
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Methylation - Lysine - Epigenetic regulation
K4 SET7/9 Hä	mflJ
ftii lamily	
Meisetz Hi	me3
SMYD family	
SMYD1 Hs	me1tf/3
5MYD3 HS	ma2/3
SET2 family	
ASH1 Dm	me3
ASH1 Hs	ms3
ASH iL Dm	me3
ASH1L Hs	rna3
SETI family	
Seil Sc	me1/2/3
SMI Sp	tt1&1 S2/3
Trithorax Dm	mel
TFR Dm	ms3
SET1A/B Hs	me3
MLL1-4 Hs	me3
ATX1 Al	m&3
K99   flr me£/3 K125 srmei K127 ßr mel
K36 SET2 1,-iini ly
SET2    Sc mel/Z/3
SET2 SETD2 ASH1 ASH1L
Sp me 1/2/3 Ms me3
Dm meS
Hs mb1/2
K43  Sf* mel K53  Wc" me2 K56  Wc- me2/3 K69  Wc" me2 K96 Wc" meS/3 K111 7f mee/3 Kiie tfc- metá
K126 Wc- mel/2 K136 We- mel
K37 Sc" m*2 Hs* me2 G^1 mtó
KS Sc- lMe
K3 JT mei/2/3 Wc" mel/2/3
met/2/3
NSD1/2 Hs mal/2 SMYD family SMYOĚ Hs mei SLTV4-20 ramlly SETD3   Or meí SUV39 family SET MAR Hs me?
K18 Hs*me1
—69 6<^
K5 nizlamity
PRDM2     Hs me?
SET2 family
ASHT        Om me3
SUV39 family
Clr4 Sp me273
Su(Vaj)3-9 Dm me3 SuV39Ht/2 Dm mal GSa/QLP   Dm me1/2
K23 Si- mel
Hs" me2 Mm" me2 Gg' me3
it me3
On m&3 Hs met/2/3 Ce inu3 Af me3
G9a/GLP SETDB1 SETDB1 Dim-S
Hs m>-\(2 Mm me3 Hs me3 Nc rrve3
Kryptonyte At me1/2
KiTvSET
EZ family
E<Z>
EZH1/2
MES-2
CURLY LEAF
SWINGER Ai me3 MEDEA    At ms3
SUV39 family
G9a Dm nwl G9a Hs mel
SET i family
ATXRS/6   Al met
K44 M5D2 me2 KSÖ        Bf meí
Sc" me2
K42 Sc1 msl/2"
K56 G9a   Hs me1
K64 Hs' ň»1
Mm' me3
K79 Dotl   Sc mů1/2/3
Dotl   Sp m*1/2/3
Dot1L Hs me 1/2/3
K122       Hs- mei
K20 3ůl9
Pr-SETT Pr-SET7
Sp mel/2/3 Dm mel Hs mel
SUV4-20 family
SUV4-2ÜH1/2HS me3
SMYD family
SMYD&        Hi me3
SETS lirtilly
NSCi Hs me3
NS02 Hs mtó/3
ASH1 Dm me3
36 Department of Experimental Biology
Mol Syst Biol. 2014 Apr 4; 10(4): 724.
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Methylation - Arginine
• Arginine can be methylated like mono- or dimethylation (Rme1 or 2) by the addition of a methyl group to its terminal side-chain £-amine.
• PRMTs can produce
o Symetrical dimethylation. o Asymetrical dimethylation.
• Arginine methylation dynamics are controlled by the regulated action of PRMTs, existence of PRDMs is controversial.
• Arginine methylation is involved in regulation of many cellular processes.
1 me trie
'-(f imelhyl-aiginifle
37 Department of Experimental Biology Yonsei Medical Journal, 2014, Vol. 55(2), p. 92 - 303
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Methylation - Arginine - Epigenetic regulation
Activation of acute myeloid leukemia genes.
H3K9me3
H4R3me2a
H3K9ac
Leukaemia target genes {e.g. HOX)
MLL fusion MOZ-TIF2
Inhibition of transcription by preventing the binding of several readers of methylated H3K4.
Repression of transcription by reducing the levels of H4K5ac.
1
H2AR3me2s-H4R3me2s, H3R8me2s
Oi
H4K5ac   ^ MYC target genes
38 Department of Experimental Biology
Nature Reviews Molecular Cell Biology, 2019, volume 20, pages 642-657.
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Methylation - Arginine - DNA-damage response
• Methylation of MRE11 by protein arginine methyltransferase 1 (PRMT1) is required for the exonuclease and resection activities of MRE11.
39 Department of Experimental Biology
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O-glycosylation
(a) O-linked
(b) N-linked
• O-linked glvcosvlation - acetylgalactosamine (GalNAc) transferase attaches GalNAc to the -OH group of a SERINE or THREONINE, also TYROSINE, in the Golgi apparatus.
• Determination of which residue is glycosylated depends on the secondary and tertiary structure.
• Usually combined oligosaccharide chains attached to an O-linked glycoprotein can contribute over 50% of the mass of a glycoprotein.
Two examples of O-linked glycoproteins:
• mucin, a component of saliva.
• ZP3, a component of the zona pellucida (which protects egg cells), if glycosylated ZP3 also acts as a sperm receptor.
40 Department of Experimental Biology
ho
c=o
GalNAc
_
Q-UDP UDP
V J
0
OCMP CMP
V J
ch,
GlcNAc
>UDP UDP
<1 O      #-GDP   GDP ? •
©
□ = N Acclylga actosaminc A = Galactose    Q = Sialic acid
=Fucosc
https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N-linked_Protein_Glycosylation_Begins_in_the_ER
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Glycosyalation
Heparan sulfate
6S
NS NS
3S
6S 6S
■2S
Proteoglycans
SHK~    y^Tl    4S    4S 4S |S I     Chondroitin or dermatan sulfate
EGF or TSR
c
to u
CT)
Ó
★ ★• So-
♦ o • 4 s o
©-4-|5orT
GPI-anchored glycoproteins
Free GAG
Hyaluronan
GlycosphingoLipids
3S
35
A Fuc	• Glc	■ GlcNAc	O Man
O Gal	^GlcA	<r IdoA	^ Sialic acid
□ GalNAc	[I GlcN	Q Inositol	
41   Department of Experimental Biology
Nature Reviews Nephrology, 2019, volume 15, pages 346-366.
SorThB O-GlcNAc rjr^y^ glycoproteins
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Lipidation
• Lipidation attachment of a lipid group, such as a fatty acid, covalently to a protein.
• In general, lipidation helps in cellular localization and targeting signals, membrane tethering and as mediator of protein-protein interactions.
Lipid modifications
• C-terminal glycosyl phosphatidylinositol (GPI) anchor
• N-terminal myristoylation
Glycine ^
A/-myristoylation
• S- and N-palmitoylation
• S-prenylation
Cysteine
42  Department of Experimental Biology
The FEBS Journal, 2022, Vol. 289, 861-882.
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C-terminal glycosylphosphatidylinositol anchor
• C-terminal glycosylphosphatidylinositol (GPI) in short, is a phosphoglyceride that can be attached to the C-terminus of a protein during posttranslational modification.
• GPI anchors tether cell surface proteins to the plasma membrane often to cholesterol- and sphingolipid-rich lipids, which act as signaling platforms on the plasma membrane.
• These protein-lipid complexes are ubiquitous in fungi, protozoans, plants, insects and animals.
• The resulting GPI-anchored proteins play key roles in a wide variety of biological processes.
o o
P = phosphate inos = inositol GlcN = glucosamine man = mannose etn = ethanolamine
Schematic GPI-anchored protein
43 Department of Experimental Biology
https://en.wikipedia.org/wiki/Glycosylphosphatidylinositol
https://www.lipidmaps.org/resources/lipidweb/lipidweb_html/lipids/complex/GPIanchor/index.htm
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C-terminal glycosylphosphatidylinositol anchor
Exterior of cell
Cytosol
t
Transmembrane protein
Lipidated protein
ŕ
GPI-anchored protein
Phospholipid
OČ"
Cholesterol
Lipid raft domain
• GPI anchors proteins to the plasma membrane are often tethered to cholesterol- and sphingolipid-rich regions called Jipid rafts".
GPI-anchored proteins function as: o receptors, transporters, and adhesion molecules o essential for the fertility of mouse sperm and egg
o coordinated growth during embryonic
development o signaling molecules to mediate cell-cell
communication o sorting signal for transport of GPI-anchored
proteins in the secretory and endocytic
pathways.
44 Department of Experimental Biology
Biochemistry 2008 47 (27), 6991-7000 https://wwwJipidmaps.org/resources/lipi^
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N-terminal myristoylation
• N-myristoylation consists of the addition of the 14-carbon fatty acid, myristate, to the N-terminal GLYCINE residue of a protein via a covalent amide bond.
• In rare cases, myristic acid is attached to a lysine (Ras GTPases and TNF) lysine myristoylation.
• N-myristoylation is catalyzed by the enzyme N-myristoyltransferase (NMT).
• Lower eukaryotes have only one isoform of NMT, whereas most mammals express two isozymes (NMT1 and NMT2).
myristoyl-CoA
Protein with an
/WWAv/\A s.CoA + H'N/YX
CH2    u N-terminal glycine
AAj-AAj-...
I
Gly,
Myristoyl-CoA: protein N-myristoyltransferases (NMT)
myristoylated protein
AAAAAA\
T
CH,
CoA-SH
AAj-AA3-
Lipids, Oct. 2020, Vol. 45(10), pages 941-6. M U 111
45 Department of Experimental Biology Cellular & Molecular Immunology, 2021, Vol. 18, pages 878-888. g Q J
N-terminal myristoylation
• N-myristoyl moiety in the protein affects, changing protein stability, influencing protein-protein interactions and enhancing subcellular targeting to organelles or the plasma membrane and so on.
• In humans, NMT isozymes, NMT1 and NMT2, are expressed in most tissues and are essential for cell survival, regulation of immune responses, and HIV-1 infection.
• N-myristoylation is considered a co-translational modification with the most accurate step occurring after the removal of the methionine initiator by methionine aminopeptidase (MetAP).
• N-myristoylation can also occur post-translationally on an internal glycine exposed by caspase cleavage during apoptosis.
46 Department of Experimental Biology
Acta Pharmacologica Sinica, 2020, Vol. 41, pages 1005-1015.
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N-terminal myristoylation
Co-translational modification: • Removal of methionine by methionine aminopeptidase (MetAP).
mRNA
aaaaa
aaaaa
aaaaa
O
mwaAn
aaaaa
NMTJ3?o
o
S-CoA V* HSCoA
Post-translational modifiction: • Internal glycine is first exposed by caspase cleavage during apoptosis.
47 Department of Experimental Biology
Acta Pharmacologica Sinica, 2020, Vol. 41, pages 1005-1015.
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N-terminal myristoylation
• LPS-induced TLR4 inflammatory responses.
• TRAM is myristoylated and anchored to the plasma membrane.
• After LPS stimulation, TLR4 dimerizes and TRAM is transiently phosphorylated by PKCs on Ser-16, which is near its N-terminus.
• TRAM dissociation from the membrane and binds to heme oxygenase-2 (HO-2), which inhibits TRAM and negatively regulating TLR4 signaling.
MUNI
48  Department of Experimental Biology Cellular & Molecular Immunology, 2021, Vol. 18, pages 878-888. r> r» t
N-terminal myristoylation
• P21-activated kinase 2 (PAK2) is cleaved by caspase 3 to produce caspase-truncated PAK2 (ctPAK2), which has a newly exposed glycine residue at the N-terminus.
• Then, NMT catalyzes the covalent attachment of myristic acid to the glycine residue of ctPAK2. Post-translationally myristoylated ctPAK2 translocates to subcellular membrane compartments to induce apoptosis.
Post-translational N-myristoylation in apoptosis
ct-PAK2 translocates to the sub-cellular membrane compartments to affect apoptosis.
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49  Department of Experimental Biology Cellular & Molecular Immunology, 2021, Vol. 18, pages 878-888. r> r» t
S-palmitoylation
S-CoA
Paimitoyl Co-A
Paimitoyl acyl transferase
SH
Cysteine residue
Pülmitoyl (hio esiemíe
Palmitoyhared cysteine residue
Palmitoylation is post-translational attachment of the saturated 16-carbon palmitate from its lipid donor, palmitovl-coenzyme A ester, to a CYSTEINE.
Paimitoyl S-acvltransferase (PATs) are enzymes responsible for catalyzing the addition of palmitate to the substrate.
Removing of palmitol by acyl-protein thioesterase (APT).
Palmitoylation is caried out on membranes, is a reversible process and several cellular proteins undergo dynamic palmitoylation.
50 Department of Experimental Biology
https://www.sciencedirect.com/topics/biochemistry-genetics-and-molecular-biology/palmitoylation
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PAT - palmitoyl S-acyltransferase
S-palmitoylation
DHHC PAT
I   II   II II
AUTOPALM ITOYLATION
PALMITATE TRANSFER
II   II   II II
U II II II
II II II II 11 II II II
Substrate
B
APT - acyl-protein thioesterase
51   Department of Experimental Biology
EMBO Reports (2018)19:e46666
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S-palmitoylation
S-palmitoylation (Cys)
N-palmitoylation
HS.
\
O-palmitoylation (Ser/Thr)     O-palmitoleoylation (Ser/Thr)
o
R = K CH3
S-Palmitovlation occurs at CYSTEINE. N-palmitovlation occurs at AM I NO-TERMINAL CYSTEINE. O-Palmitovlation and O-palmitoleoylation occur at SERINE/THREONINE.
Protein acyl transferases are located:
• Endoplasmic reticulum
• Golgi apparatus
• Plasma membrane
Cell Chem Biol, Volume 25, Issue 3, 15 March 2018, Pages 236-246. M U 111
52  Department of Experimental Biology ^ _ _
^ ay The FEBS Journal, 2022, Vol. 289,861-882. O p T
S-prenylation
• S-prenylation, similarly to S-palmitoylation, provides a hydrophobic, membrane attracted C terminus through the enzymatic addition of farnesyl (C15) or geranylgeranyl (C20) to a CYSTEINE residue.
• Enzyme involved in this reaction is farnesyl transferase (FT) or geranylgeranyl transferases (GGTIand II).
• Dysregulated S-prenylation is implicated in several diseases including cancer.
o
protein—MH-C
myistoylated protein
O
protein—S—ü^
palmitoylated protein
pren^lated protein
protein—S-
53 Department of Experimental Biology https://www.mun.ca/biology/scarr/iGen3_06-08.html
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Proteolytic cleavage
• Proteolytic cleavage - very common irreversible post-translational modification of the protein's structure and biological function.
• Also, first amino acid methionine of a newly synthesized polypeptide is very often cleaved off (also true for some prokaryotic f-Met).
• The precursor protein is termed a proprotein, and the peptide that is cleaved off proprotein is called the propeptide.
• Classical examples of proproteins are the hormone insulin, the cell death protein family of caspases, collagen and the Alzheimer-associated neural protein (3-amyloid.
https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N-Department of Experimental Biology iinked_Protein_Glycosylation_Begins_in_the_ER
Chem. Rev. 2018, 118, 3, 1137-1168.
Proteolytic cleavage
In mammals - preproinsulin (inactive as a hormone) is first translated from the insulin mRNA.
Proteolytic processing is necessary to make biologically active insulin.
(A) The linear protein contains a signal sequence, which is cleaved (1) after the protein enters the ER, an A chain, a B chain, and a C-peptide.
(B) Inside the ER, the proinsulin (insulin precursor) folds and disulfide bonds form between cysteines.
(C) Finally, two cleavages (2,3) release the C peptide, which leaves the A and B chains attached by the disulfide bonds. This is now active insulin.
B chain-__
C-peptide
£lQ   K-R-G-l-V-E-Q-C-C-T-S -i-C-S-L-Y-Q-L-E N Y-C-N
J..
_
r-V-VQ-H L C GS H L V-E -A-L-Y-L-V C G-E-R -G-F-F-Y-T-P-K-T
AchairK SH
i-1
S S
i-1-1-,
I K-R-G-l-V-E-Q-C-C-T-S+C-S-L-YQL-E-N-Y-C-N I
I F-VN-Q-H-LCG-SHL-V-E-A-L-Y-LV<GE-RG-f F-Y-TPKT I
55 Department of Experimental Biology
https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N-linked_Protein_Glycosylation_Begins_in_the_ER
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Proteolytic cleavage
OH
Procollagen H2N
COOH
OH
OH
Propeptide
J
Completed collagen molecule
Propeptide Triple helix formation
Secretion from cell Propeptides clipped
Collagen is a very large secreted protein, twisted triple-helix of three subunit, that provides structure and shock absorbance for the extracellular matrix in animals.
The collagen subunits are made as procollagen, and propeptides are lopped off of both N- and C-termini to generate the final protein.
However, they are not cleaved off until after the three subunits assemble around one another.
The propeptide sequences are clearly necessary for efficient assembly of the final protein complex.
56 Department of Experimental Biology
https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N-linked_Protein_Glycosylation_Begins_in_the_ER
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DNA
Precursor i protein
Spliced protein
N-extein
N-extein
N-extein
intein
C-exlein
Transcrlptřon/translahon intein C-extein
Protein splicing C-extein intein
Protein splicing
Protein splicing is a post-translational process facilitated by an intervening polypeptide, called an intein (for internal protein).
The intein interrupts flanking polypeptides called exteins.
The intein is responsible for catalyzing its excision from the exteins, concomitant with extein ligation.
N-axtoin
Inlein frocKs:
H
Tis.'I
Hciming Bndonudsase Irrinin _
Ď II
i;
5.T
C □ E
F G
• Inteins have four conserved sequence blocks. Block C, D and E where the split sites of naturally occurring split inteins and homing endonuclease domain (HED) are located.
57 Department of Experimental Biology
Handbook of Proteolytic Enzymes, Volume 1, 2013, Pages 315-321
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DNA
Exon 1  Intron  Exon 2
Protein splicing
TRANSCRIPTION
RNA
TRANSCRIPTION
The protein splicing is rare PMT
on 1  Intron  Exon 2 Extein 1 Intein Extein 2
SPLICING OF RNA
mRNA Exort 1 Exon 2
TRANSLATION
TRANSLATION
PROTEIN
Fi J1"!
From exon 1 jnlejn
From ^extein 1
From
extein 2
SPLICING OF PROT ESN
58 Department of Experimental Biology
• Inteins and exteins are the protein analogs of the introns and exons found in the DNA and RNA. In other words, inteins are intervening sequences in proteins that are present when the protein is first made, but are later spliced out.
• The final protein is made of the exteins that are now joined together.
• Inteins have been found in yeasts, algae, bacteria, and archaea (archaebacteria), such as VMA1 in a precursor of a vacuolar H+-ATPase enzyme.
https://www.sciencedirect.com/topics/biochemistry-genetics-and-molecular-biology/protein-splicing
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Protein splicing
Protein splicing is four-step process, which is achieved through structural conformational change and chemical bonds shifting on junction sites between intein and exteins.
1. A nucleophilic displacement converts the peptide bonding to an ester or thioester group.
2. Transesterification - transfers the to the first residue of C-extein, forming a branched intermediate.
3. The Asn cvclization leads to intein peptide bond cleavage and exteins ligation.
4. Rapid conversion from the ester bond to the amide bond occurs to form the final peptide.
April 2013Molecules 18(1):440-65 Department of Experimental Biology Front Bjoeng Biotechno| 2022, Protein Splicing of Inteins: A Powerful Tool in Synthetic
Biology, 10:810180
Protein splicing
Chrůmosůme with spíil dnäE gene
DNA     Exiein 1 tnteln 1
Mein 2 Extein
The DNA coding for the DnaE protein of Synechocystis is transcribed and translated into two separate proteins, each containing an intein and an extein.
The exteins of the two proteins are spliced together by the inteins. During splicing both inteins are lost.
Also, DnaE, the catalytic subunit a of DNA polymerase III, is encoded by two separate genes, dnaE-n and dnaE-c.
TRANSCRIPTION AND TRANSLATION
PRE-PROTEIN
Xi^j/L Intein ^ i- -,-.-..1-, i
PROTEIN
Intein 1 Intein 2 * \^
Extein 2
I
t        *^ Extein Extein 1
Intein 1
intein 2
60 Department of Experimental Biology
https://www.sciencedirect.com/topics/biochemistry-genetics-and-molecular-biology/protein-splicing
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Post-translational Ubiquitination
• Ubiquitin (Ub), a highly conserved regulatory protein containing 76 amino acids, can be covalently tagged to target proteins.
• Ubiquitin is attached to the LYSINE residue in polypeptide.
• Ubiquitin provides eight types of polyubiquitin linkages (K6, K11, K27, K29, K33, K48, K63 and Met1) with specific functions.
• The ubiquitin ligase adds ubiquitin to the substrate and deubiquitilating enzyme removes Ub from the substrate. Thus, ubiquitination is reversible process.
61   Department of Experimental Biology
Mater methods, 2014;4:827
Physiological Reviews. Jul 2013, 93(3):1289-315.
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(Ob) Ubiquitin ~ Thioester bond O AMP * Lys
A Catalytic Cys
®
Mg2\ ATP
Post-translational Ubiquitination
• Ubiquitin can be covalently tagged to target proteins via a cascade of enzymatic reactions.
• 1. A ubiquitin-activating enzyme (E1) catalyzes binding to one ubiquitin by a thioester.
• 2. E1 then binds a ubiquitin-conjugating enzyme (E2) and transfers ubiquitin from its catalytic cysteine to the catalytic cysteine of E2 to form E2—ubiquitin (~ indicates a thioester bond).
• 3. A ubiquitin ligase (E3) recruits E2—ubiquitin and a substrate to catalyze ubiquitin transfer to a lysine on the substrate.
62  Department of Experimental Biology
Nature Reviews Molecular Cell Biology, 2016, Volume 17, pages 626-642.
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Post-translational Ubiquitination
o
li
-c-o
Ubiquitin activating enzyme ~2 Uba1 Ubae
O
-SH-
ATP
AMP+PPi
Ubiquitin conjugating enzyme -20
Ubiquitin ligase -600
HECT E3 ligase RING E3 ligase
_BJ3_jQ—-e
3
F-box
Three distinct classes of ubiquitin ligases. o HECT E3 o RING/U-box E3 o RBR E3.
These ubiquitin ligases utilize different structural mechanisms for mediating the final transfer of ubiquitin onto substrates.
IBR
63 Department of Experimental Biology
[dub]
_C—|NJH —(^SubJ   Deubiquitinases-100
Signal Transduction and Targeted Therapy (2020) 5:11.
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Post-translational Ubiquitination
Protein could be: o Monoubiquitylated.
o Multi-monoubiquitylated.
o Polyubiquitylated.
o Branched ubiquitin chain
Monoubiquitylation Multi-
monoubiquitylation
Homotypic chains
Mixed
Branched
K48
KG
Heterotypic chains
64 Department of Experimental Biology
Physiological Reviews. Jul 2013, 93(3):1289-315. Cell Discovery volume 7, Article number: 6 (2021)
Post-translational Ubiquitination
Branched ubiquitin chains of different topologies are specialized for different cellular functions and control the stability, activity, interaction properties, and localization of many different proteins.
Branched ubiquitin chains regulate cell signaling and protein degradation pathways.
Branched ubiquitin chains are remarkably diverse in terms of their chemical linkages, structures, and the biological information they transmit.
Lys48
Monoubiquitylation or multi-mono ubiquitiylation
Lys63
Polyubiquitylation chains
Lys48-linked polyubiquitin
Lys63-linked polyubiquitin
• DNA repair
• Transcription
• Trafficking
• Endocytosis
1 26S proteasome   • DNA repair, degradation        • NFkB signalling
• Trafficking
• Endocytosis
Jb) Ubiquitin ~ Thioester bond O AMP * Lys
A Catalytic Cys
Branched ubiquitin chain
> APC/C-catalysed 26S proteasome degradation
Nature Reviews | Molecular Cell Biology
65 Department of Experimental Biology
Nature Reviews Molecular Cell Biology, 2016, Volume 17, pages 626-642.
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Post-translational Ubiquitination
Model for the role of branched K48/K63 chains in the activation of NF-kB signaling.
Homotypic K63-linked chains are efficiently disassembled by CYLD, resulting in the removal of K63 linkages from TRAF6 and the termination of NF-kB signaling.
Homotypic K63 chain
® ® © @
TRAF6
Termination of NF-kB signaling
Branched K48/K63 chain
66 Department of Experimental Biology
Sustained NF-kB signaling
Branched K48/K63 chains are resistant to CYLD cleavage, resulting in the persistence of K63 linkages on TRAF6 and sustained activation of NF-kB signalling.
Cell Discovery volume 7, Article number: 6 (2021)
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Ubiquitin-proteasome system
Ubiquitination
atp +p;pí fa Q
26S proteasome
HECTE3
19S
20S
19S
c
O
03 TD 03
CD CD "Ö
"03
E o
CO 03 CD
•4—'
2 o_
o
TO CT
CD Q
Ubiquitin recycling
67 Department of Experimental Biology
Lys11-Cell cycle regulation Lys27-Mitophagy Lys48-Proteasomal degradation Lys63-NFKB singnaling Endocytosis
https://www.antibody-creativebiolabs.com/post-translational-modification-ptm.htm
The overall system of ubiquitination and proteasomal degradation is known as the ubiquitin-proteasome system.
Ubiquitination is covalently conjugated to a Lysine residue of the substrate proteins.
Lys48-linked polyubiquitin chains usually target proteins for proteasomal degradation.
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Ubiquitin-proteasome system
The proteasome is a multi-catalytic molecular machine that plays a key role in the degradation of many cytoplasmic and nuclear proteins.
The core of the proteasome consists of a symmetrical cylinder-shaped structure composed of four stacked rings, each containing 7 different subunits and is called the 20S proteasome.
Gate opening of the 20S core occurs via capping by proteasome activators such as the 19S cap or PA28.
The 19S cap is the most abundant activator and it forms the 26S proteasome together with the 20S core.
Latent 20S
Immunoproteasome
Department of Experimental Biology
Front. Mol. Biosci. 6:56., doi: 10.3389/fmolb.2019.00056
Ubiquitin-proteasome system
Substrate processing by the 26S proteasome
polyubiquitin
chain substrate
<-> I-, 2-25 residue 1_ _f peptides
/
antigenic peptides    amino acids
69 Department of Experimental Biology
• The 26S proteasome is a 2.4-MDa molecular machine that makes up nearly 2% of total cellular protein.
• It is composed of a 20S proteasome core particle capped on one or both ends by the 19S regulatory particle.
• It degrades proteins by a multistep process; the 19S regulatory particle binds ubiquitinated substrates, opens a substrate entry gate in 20S and unfolds its substrates by linearly translocating them into the 20S catalytic chamber, where they are degraded to peptides.
MUNI
Pharmacological Reviews April 2019, 71 (2) 170-197
Post-translational Ubiquitination
• The enhanced binding of branched chains to the 19S regulatory particle of proteasome as a result of an increase in the local concentration or "density" of ubiquitin subunits surrounding the substrate is illustrated by the multivalent-binding model.
• Enhanced binding due to the recognition of novel interaction surfaces created by branching or recognition of the branch point itself is represented by the conformational recognition model.
19S regualtory particle
70 Department of Experimental Biology
Cell Discovery volume 7, Article number: 6 (2021)
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Sumolyation
• Sumoylation is a post-translational modification, Small Ubiquitin-like Modifier (or SUMO) proteins are a family of small proteins that are covalently attached to and detached from other proteins in cells to modify their function.
• Sumoylation is reversed by the action of desumoylating enzymes.
• Here are 4 confirmed SUMO isoforms in humans; SUMO-1, SUMO-2, SUMO-3 and SUMO-4.
• SUMO proteins are small; most are around 100 amino acids in length and 12 kDa in mass.
• SUMO protein has a unique N-terminal extension of 10-25 amino acids which other ubiquitin-like proteins do not have.
MUNI
71   Department of Experimental Biology https://en.wikipedia.org/wiki/SUMO_protein
O 0 J.
Sumolyation
• First, SUMO (S) is matured by SUMO specific proteases (Prot), enabling it to become activated in an ATP-consuming reaction, to form a thioester bond (-S-) with the heterodimeric E1 (Aos1/Uba2).
• SUMO is then transferred to the E2 (Ubc9), resulting in a thioester bond.
• Finally, SUMO is conjugated directly or with the help of an E3 ligase to its substrate, forming an isopeptide bond.
• Sumoylation is reversed by SUMO specific proteases that cleave SUMO from the substrate.
72  Department of Experimental Biology
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Sumolyation
Deconjugation
SUMO proteases
SUMO proteases (nine in human)
c .0
"■I—I
CO
3 +
- V  w ATP
SUMO     ► +
precursor
i ik n AMP Uba2 +ppi
Aos1
s
Monosumoylation
Polysumoylation
Multisumoylation
Substrates
E2
conjugating (one)
E1 E3 activating ligating (one) (ten in human) (thousands)
Conjugation
Enzymes in sumolyation o E1 - 1 o E2- 1 o E3-10
Substrates can be: o Monosumoylation o Multisumoylation o Polysumoylation.
73 Department of Experimental Biology
BioMol Concepts 2017; 8(1): 13-36.
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Sumolyation
• Sumoylation is involved in various cellular processes, such as nuclear-cytosolic transport, transcriptional regulation, apoptosis, protein stability, response to stress, and progression through the cell cycle by one of these mechanisms:
Alters substrate Regulation of substrate Promotes Blocks
conformation stability through recruitment of interactions interactions
SUMO-targeted ubiquitin ligases
Department of Experimental Biology Physiol Rev94: 1249-1285, 2014doi:10.1152/physrev.00008.2014
• Protein folding and Quality control
MUNI
75 Department of Experimental Biology _ _ T
O U J.
Protein folding
• Protein folding is the physical process by which a linear polypeptide folds into its characteristic and functional three-dimensional structure.
• The final folded configuration, or shape, of a protein is determined by its amino acid sequence.
• Protein folding is also strongly influenced by the solubility of the AA R-groups in water.
• Protein can reach its 3D conformation either alone, co-translational folding, or with help of other factors, chaperones.
Unfolded Folded
https://slidetodocxom/protein-folding-the-production-of-a-mature-protein/ |j
Conference: 2016 IEEE 2nd International Foru Industry Leveraging a better tomorrow (RTSI)
76 Department of Experimental Biology Conference: 2016 IEEE 2nd International Forum on Research and Technologies for Society and g Q J
Protein folding
Hydrophobic versus hydrophilic characteristic of AA.
Three types of noncovalent bonds help proteins to fold.
polar
side chains
nonpolar side chains
hydrophobic core region contains nonpolar side chains
polar side chains on the outside of the molecule can form hydrogen bonds to water
unfolded polypeptide
folded conformation in aqueous environment
hydrogen bond
77 Department of Experimental Biology
https://slidetodoc.com/protein-folding-the-production-of-a-mature-protein/
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Co-translational protein folding
• Protein domains can fold into stable tertiary structures while they are synthesized by the ribosome in a process known as co-translational folding. Folding begins early inside the polypeptide exit tunnel.
• The nascent chain (NC) emerging from the ribosome can interact with chaperones, biogenesis factors, or other proteins.
NC starts to fold vectorially Secondary structures can form NC interacts with the exit tunnel
NC can compact to tertiary structures
Ribosome surface destabilizes folding intermediates and ensures correct timing of folding for single- and multi-domain proteins
NC can interact with its partner subunits of an
oligomeric complex, chaperones or biogenesis
factors
78 Department of Experimental Biology
Biomolecules 2020, Cotranslational Folding of Proteins on the Ribosome, 10(1), 97.
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Protein folding
* The ER lumen plays four major protein processing roles:
o folding/refolding of the polypeptide, o glycosylation of the protein, o assembly of multi-subunit proteins o packaging of proteins into vesicles.
CS='
Q Quoose    <^ BiP A Ubiquitin    Ö Ribosome V Tmnstoccn O COPil
Nature Reviews | Molecular Cell Biology
79 Department of Experimental Biology
https://bio.libretexts.org/Bookshelves/Cell_and_Molecular_Biology/N-
linked_Protein_Glycosylation_Begins_in_the_ER
https://www.sciencedirect.com/science/article/pii/S1568163709000178
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Protein folding
• If there is incorrect bound between cysteines, and more stable cysteines bond in the context of the whole protein is available, than the exchange of disulfide bonding is catalyzed by protein disulfide isomerase (PDI).
• This enzyme uses a sulfhydryl group of a cysteine residue as temporary bonding partner in order to break disulfide bonds on the target protein and allow for new ones to form.
• Note that the formation of a new bond is not directed by PDI, but is instead a stochastic process in which a stronger binding partner displaces the PDI —SH.
A
B
C
D
80 Department of Experimental Biology
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Chaperones
Protein folding take place in the cytosol.
Most proteins require the assistance of molecular chaperones.
Bacteria
(Hsp70) (Hsp40)
Oltet chapflfDfws
GroEL
+ GrpE. ATP * LJNEF)
20
+ ATP
Althaea
i T)H?rrnůson»
Eukarya
NAC
MAC
RAC
Hsp40ťIL FtAC Hep40 HSp70| hrSpTOj
syslem <gj
-20 %
NEFs ATP
TflJC
81   Department of Experimental Biology
Cold Spring Harb Perspect Biol 2010;2:a004390
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Chaperones
• The heat-shock proteins (Hsp) are a family of molecular chaperones, which collectively form a network that is critical for the maintenance of protein homeostasis.
• Most proteins require the assistance of molecular chaperones, like Hsp 70 & Hsp 60, to reach their final folded form.
• Hsp 70 and Hsp 60 act sequentially on proteins to help them achieve their correct folded state.
• Proteins that fail to be properly folded are ultimately targeted for destruction.
82  Department of Experimental biology
Molecular Biology, 430 (22), 4525-4546
https://slidetodoc.com/protein-folding-the-production-of-a-mature-protein/
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Chaperones
• Molecular chaperones, like those in the Hsp 60 and Hsp 70 families, help guide the folding of most newly-synthesized proteins.
• Hsp chaperones bind to hydrophobic patches that are exposed on incompletely folded proteins.
• Repeated cycles of ATP binding and hydrolysis are generally required for the proper folding of a polypeptide chain.
protein
83 Department of Experimental biology
https://slidetodoc.com/protein-folding-the-production-of-a-mature-protein/
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Chaperones
• Hsp 60 acts on fully-synthesized proteins that have not yet achieved their final folded form.
• The presence of incompletely folded proteins can lead to the formation of aggregates that may have dangerous consequences for the cell.
hspbOliko protein complex
84 Department of Experimental Biology
https://slidetodoc.com/protein-folding-the-production-of-a-mature-protein/
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Chaperones
Hsp70/40 mediates the initial stages of protein folding and acts as a central hub in the Hsp chaperone network.
If Hsp70/40 is only able to partially fold the protein, it can be transferred to either the Hsp90 or Hsp60 systems in order to acquire a folded functional conformation.
Cellular stress conditions can cause proteins to misfold and associate into insoluble, toxic aggregates.
Physiological conditions Ribosome
Cellular stress conditions
Hsp70/40
85 Department of Experimental biology
Molecular Biology, 430 (22), 4525-4546
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Chaperones
crisp* rone Family      Topology of anal 119			Known Function
HsplM	Ö 0	app.stpe. Htp70.H!p40	* Wofkawith DnaK in rVrP-depandBM disaggregation and prc!aa!ya=a * Prevent aggregariorvdagradolicfland turnover onnMerrtblnd mtMhOndrial proteins +    Reactivates haa^a rrraged arolem* * Establiahea and maintains prion phanolype in yaas<
mm		Hop, Hip. W.pTO. Iromunophlllni,	• R«j(c)ld«pfotain»inftra«MdcHS Pnobablt wciKloryenaparonaiin prokaryatea • Major cytosolic chapanona in eukaryotea. • CytDprotactionand fnrjacellulaf signaling • In Eft, conlrelsprcteifl nomeostasi*. folding and'aajsmbt^oi' *«««fory
HspTC		Hr;p40.Grp£	* Ubi^uiraua Principal folding chaparora * Worts with CIpS as dtsaggiegoM ♦ Folding of newly synthas^ad prolemt ♦ Prcflesnlnanapflrl into ER and mflechondnn
H:--■' ■ (0 roupi}	i$ j iii 00		«   Major chaperone forprcrtain folding in prokaryatas • StsDiliat protaia»<H*ing Mat *Wtt • Pfc«*ioWt fgldmg of ovarnpro^ucedprOltani • Major chaperoneinmrtoenondna and chloropusl
HspfO (Croup :i|		FTafc;. - z ■:	*    Prc.nro:fis (aiding of a e^pai} c rjujiemi m aukaryole* '    Re1o dine oF unfolded polypaplicf*s,nvlro
	'-Oř	-	* StobiliMt unfdd*d polffjiptri** * PrBvejiiaarjgregaiJEn * Werta-Aith HapTOin pralatri fafclding. * StnwIuraJ protain 0! eye, lena
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86 Department of Experimental biology
Quality control of protein synthesis
• Because proteins are structurally dynamic, constant surveillance of the proteome by an integrated network of chaperones and protein degradation machineries is required to maintain protein homeostasis (proteostasis).
newly
synthesized protein
protein aggregate
correctly folded correctly folded incompletely without help     with help of a     folded forms
molecular digested by the increasing time                               chaperone proteasome
Figure 6-88 Molecular Biology of the Cell (© Garland Science 2008)
87 Department of Experimental biology
https://slidetodoc.com/protein-folding-the-production-of-a-mature-protein/
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Quality control of protein synthesis
• Chaperones also cooperate with other components of the proteostasis network, such as the proteasome system and autophagy, in the removal of terminally misfolded and aggregated proteins through proteolytic degradation.
Key:
—► Promoted by chaperones —► Off-pathway interactions
_II_II_II_
Folding Conformational Aggregate Clearance by
maintenance formation degradation
88 Department of Experimental biology
Science, Jul 2016 , Vol. 353, issue 6294.
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Protein Misfolding Diseases
• Many inherited diseases result from mutant proteins that evade quality control processes, fold abnormally and ultimately form aggregates.
• The gradual decline of protein quality controls with age can also lead to disease by permitting normal proteins to form misfolded protein aggregates that can
impair cellular functions.
Protein misfolding diseases:
• Huntington's
• Alzheimer's
• Parkinson's
• aggregates in patients can be intracellular or extracellular.
89 Department of Experimental biology
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Post-translational modifications in histones
PTM events mediate diverse biological functions such as transcriptional activation and inactivation, chromosome packaging, and DNA damage and repair processes.
■e Acotyl.ition ^ Mothylation £ Phosphorylation Q Ubiquitination
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90 Department of Experimental biology
https://www.thermofisher.com/cz/en/home/life-science/protein-biology/protein-biology-learning-center/protein-biology-resource-library/pierce-protein-methods/overview-post-translational-modification.html
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Post-translational modifications in cell signaling
PDGF
FGF2 IGF
HTK
HTK
RAS RAF
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PIPS —i. POKt
W
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91   Department of Experimental biology
PROLIFERATION
March 2017Pulmonary Circulation 7(2):204589321770143
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THANK YOU FOR YOUR ATTENTION
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