Integrin: Difference between revisions

Integrin alpha cytoplasmic region
Structure of chaperone protein PAPD.[1]
Identifiers
Symbol	Integrin_alpha
Pfam	PF00357
InterPro	IPR000413
PROSITE	PDOC00215
SCOP2	1dpk / SCOPe / SUPFAM
OPM superfamily	197
OPM protein	2knc
Available protein structures: Pfam   structures / ECOD   PDB RCSB PDB; PDBe; PDBj PDBsum structure summary PDB 1dpk​, 1dpq​, 1kup​, 1kuz​, 1m8o​, 1s4w​

Integrin alpha
Structure of the extracellular segment of integrin alpha Vbeta3.[2]
Identifiers
Symbol	Integrin_alpha2
Pfam	PF08441
Pfam clan	CL0159
InterPro	IPR013649
SCOP2	1jv2 / SCOPe / SUPFAM
Available protein structures: Pfam   structures / ECOD   PDB RCSB PDB; PDBe; PDBj PDBsum structure summary PDB 1jv2​, 1l5g​, 1m1x​, 1u8c​

Integrin, beta chain
Identifiers
Symbol	Integrin_beta
Pfam	PF00362
InterPro	IPR002369
SMART	SM00187
PROSITE	PDOC00216
SCOP2	1jv2 / SCOPe / SUPFAM
Available protein structures: Pfam   structures / ECOD   PDB RCSB PDB; PDBe; PDBj PDBsum structure summary PDB 1jv2​, 1kup​, 1kuz​, 1l3y​, 1l5g​, 1m1x​, 1m8o​, 1s4x​, 1txv​, 1ty3​, 1ty5​, 1ty6​, 1ty7​, 1tye​, 1u8c​

Integrin beta cytoplasmic domain
crystal structure of the filamin a repeat 21 complexed with the integrin beta7 cytoplasmic tail peptide
Identifiers
Symbol	Integrin_b_cyt
Pfam	PF08725
InterPro	IPR014836
SCOP2	1m8O / SCOPe / SUPFAM
Available protein structures: Pfam   structures / ECOD   PDB RCSB PDB; PDBe; PDBj PDBsum structure summary

Integrin beta tail domain
crystal structure of the extracellular segment of integrin alphavbeta3
Identifiers
Symbol	Integrin_B_tail
Pfam	PF07965
InterPro	IPR012896
SCOP2	1jv2 / SCOPe / SUPFAM
Available protein structures: Pfam   structures / ECOD   PDB RCSB PDB; PDBe; PDBj PDBsum structure summary

Integrins are receptors that mediate the attachment between a cell and the tissues that surround it, such as other cells or the extracellular matrix (ECM). In signal transduction, integrins pass information about the chemical composition of the ECM into the cell. Therefore, they are involved in cell signaling and the regulation of cell cycle, shape, and motility.

Typically, receptors inform a cell of the molecules in its environment and the cell responds. Not only do integrins perform this outside-in signaling, but they also operate an inside-out mode. Thus, they transduce information from the ECM to the cell as well as reveal the status of the cell to the outside, allowing rapid and flexible responses to changes in the environment, for example to allow blood coagulation by platelets.

There are many types of integrin, and many cells have multiple types on their surface. Integrins are of vital importance to all animals and have been found in all animals investigated, from sponges to mammals. Integrins have been extensively studied in humans.

Integrins work alongside other proteins such as cadherins, immunoglobulin superfamily cell adhesion molecules, selectins and syndecans to mediate cell–cell and cell–matrix interaction and communication. Integrins bind cell surface and ECM components such as fibronectin, vitronectin, collagen, and laminin.

Structure

Integrins are obligate heterodimers containing two distinct chains, called the α (alpha) and β (beta) subunits. In mammals, eighteen α and eight β subunits have been characterized, whereas the Drosophila genome encodes only five α and two β subunits, and Caenorhabditis nematodes possess genes for two α subunits and one β.^[3] The α and β subunits each contain two separate tails, both of which penetrate the plasma membrane and possess small cytoplasmic domains.^[4]Template:Multicol alpha

gene	protein	synonyms are
ITGA1	CD49a	VLA1
ITGA2	CD49b	VLA2
ITGA3	CD49c	VLA3
ITGA4	CD49d	VLA4
ITGA5	CD49e	VLA5
ITGA6	CD49f	VLA6
ITGA7	ITGA7	FLJ25220
ITGA8	ITGA8
ITGA9	ITGA9	RLC
ITGA10	ITGA10
ITGA11	ITGA11	HsT18964
ITGAD	CD11D	FLJ39841
ITGAE	CD103	HUMINAE
ITGAL	CD11a	LFA1A
ITGAM	CD11b	MAC-1
ITGAV	CD51	VNRA, MSK8
ITGAW	ITGAW
ITGAX	CD11c

Template:Multicol-break beta

gene	protein	synonyms
ITGB1	CD29	FNRB, MSK12, MDF2
ITGB2	CD18	LFA-1, MAC-1, MFI7
ITGB3	CD61	GP3A, GPIIIa
ITGB4	CD104
ITGB5	ITGB5	FLJ26658
ITGB6	ITGB6
ITGB7	ITGB7
ITGB8	ITGB8

Template:Multicol-end

In addition, variants of some of the subunits are formed by differential splicing; for example four variants of the beta-1 subunit exist. Through different combinations of these α and β subunits, some 24 unique integrins are generated, although the number varies according to different studies.^[5]

Integrin subunits span the plasma membrane and in general have very short cytoplasmic domains of about 40–70 amino acids. The exception is the beta-4 subunit, which has a cytoplasmic domain of 1088 amino acids, one of the largest known cytoplasmic domains of any membrane protein. Outside the cell plasma membrane, the α and β chains lie close together along a length of about 23 nm; the final 5 nm N-termini of each chain forms a ligand-binding region for the extracellular matrix (ECM).

The molecular mass of the integrin subunits can vary from 90 kDa to 160 kDa. Beta subunits have four cysteine-rich repeated sequences. Both α and β subunits bind several divalent cations. The role of divalent cations in the α subunit is unknown, but may stabilize the folds of the protein. The cations in the β subunits are more interesting: they are directly involved in coordinating at least some of the ligands that integrins bind.

There are various ways of categorizing the integrins. For example, a subset of the α chains has an additional structural element (or "domain") inserted toward the N-terminal, the alpha-A domain (so called because it has a similar structure to the A-domains found in the protein von Willebrand factor; it is also termed the α-I domain). Integrins carrying this domain either bind to collagens (e.g. integrins α1 β1, and α2 β1), or act as cell-cell adhesion molecules (integrins of the β2 family). This α-I domain is the binding site for ligands of such integrins. Those integrins that don't carry this inserted domain also have an A-domain in their ligand binding site, but this A-domain is found on the β subunit.

In both cases, the A-domains carry up to three divalent cation binding sites. One is permanently occupied in physiological concentrations of divalent cations, and carries either a calcium or magnesium ion, the principal divalent cations in blood at median concentrations of 1.4 mM (calcium) and 0.8 mM (magnesium). The other two sites become occupied by cations when ligands bind—at least for those ligands involving an acidic amino acid in their interaction sites. An acidic amino acid features in the integrin-interaction site of many ECM proteins, for example as part of the amino acid sequence Arginine-Glycine-Aspartic acid ("RGD" in the one-letter amino acid code).

High resolution structure

Despite many years of effort, discovering the high-resolution structure of integrins proved to be challenging: membrane proteins are classically difficult to purify, and integrins are also large, complex and linked to many sugar trees ("highly glycosylated"). Low-resolution images of detergent extracts of intact integrin GPIIbIIIa, obtained using electron microscopy, and even data from indirect techniques that investigate the solution properties of integrins using ultracentrifugation and light scattering, were combined with fragmentary high-resolution crystallographic or NMR data from single or paired domains of single integrin chains, and molecular models postulated for the rest of the chains.

Despite these wide-ranging efforts, the X-ray crystal structure obtained for the complete extracellular region of one integrin, αvβ3, was a surprise.^[6] It showed the molecule to be folded into an inverted V-shape that potentially brings the ligand-binding sites close to the cell membrane. Perhaps more importantly, the crystal structure was also obtained for the same integrin bound to a small ligand containing the RGD-sequence, the drug cilengitide.^[7] As detailed above, this finally revealed why divalent cations (in the A-domains) are critical for RGD-ligand binding to integrins. The interaction of such sequences with integrins is believed to be a primary switch by which ECM exerts its effects on cell behaviour.

The structure poses many questions, especially regarding ligand binding and signal transduction. The ligand binding site is directed towards the C-terminal of the integrin, the region where the molecule emerges from the cell membrane. If it emerges orthogonally from the membrane, the ligand binding site would apparently be obstructed, especially as integrin ligands are typically massive and well cross-linked components of the ECM. In fact, little is known about the angle that membrane proteins subtend to the plane of the membrane; this is a problem difficult to address with available technologies. The default assumption is that they emerge rather like little lollipops, but the evidence for this sweet supposition is noticeable by its absence. The integrin structure has drawn attention to this problem, which may have general implications for how membrane proteins work.

Although the crystal structure changed surprisingly little after binding to cilengitide, the current hypothesis is that integrin function involves changes in shape to move the ligand-binding site into a more accessible position, away from the cell surface, and this shape change also triggers intracellular signaling. There is a wide body of cell-biological and biochemical literature that supports this view. Perhaps the most convincing evidence involves the use of antibodies that only recognize integrins when they have bound to their ligands, or are activated. As the "footprint" that an antibody makes on its binding target is roughly a circle about 3 nm in diameter, the resolution of this technique is low. Nevertheless, these so-called LIBS (Ligand-Induced-Binding-Sites) antibodies unequivocally show that dramatic changes in integrin shape routinely occur. However, how the changes detected with antibodies look like on the structure is still unknown.

Activation

When released into the cell membrane, newly synthesized integrin dimers are speculated to be found in the same "bent" conformation revealed by the structural studies described above. One school of thought claims that this bent form prevents them from interacting with their ligands, although bent forms can predominate in high-resolution EM structures of integrin bound to an ECM ligands. Therefore, at least in biochemical experiments, integrin dimers must apparently not be 'unbent' in order to prime them and allow their binding to the ECM. In cells, the priming is accomplished by a protein named Talin, which binds to the β tail of the integrin dimer and changes its conformation.^[8][9] Moreover, talin proteins are able to dimerize^[10] and thus are thought to intervene in the clustering of integrin dimers which leads to the formation of a focal adhesion. Recently, the Kindlin-1 and Kindlin-2 proteins have also been found to interact with integrin and activate it.^[11]

Function

Integrins have two main functions:

• Attachment of the cell to the ECM
• Signal transduction from the ECM to the cell

However, they are also involved in a wide range of other biological activities, including immune patrolling, cell migration, and binding to cells by certain viruses, such as adenovirus, echovirus, hantavirus, and foot and mouth disease viruses.

A prominent function of the integrins is seen in the molecule GPIIbIIIa, an integrin on the surface of blood platelets (thrombocytes) responsible for attachment to fibrin within a developing blood clot. This molecule dramatically increases its binding affinity for fibrin/fibrinogen through association of platelets with exposed collagens in the wound site. Upon association of platelets with collagen, GPIIbIIIa changes shape, allowing it to bind to fibrin and other blood components to form the clot matrix and stop blood loss.

Attachment of cell to the ECM

Integrins couple the ECM outside a cell to the cytoskeleton (in particular the microfilaments) inside the cell. Which ligand in the ECM the integrin can bind to is defined by which α and β subunits the integrin is made of. Among the ligands of integrins are fibronectin, vitronectin, collagen, and laminin. The connection between the cell and the ECM may help the cell to endure pulling forces without being ripped out of the ECM. The ability of a cell to create this kind of bond is also of vital importance in ontogeny.

Cell attachment to the ECM is a basic requirement to build a multicellular organism. Integrins are not simply hooks, but give the cell critical signals about the nature of its surroundings. Together with signals arising from receptors for soluble growth factors like VEGF, EGF, and many others, they enforce a cellular decision on what biological action to take, be it attachment, movement, death, or differentiation. Thus integrins lie at the heart of many cellular biological processes. The attachment of the cell takes place through formation of cell adhesion complexes, which consist of integrins and many cytoplasmic proteins such as talin, vinculin, paxillin, and alpha-actinin. These act by regulating kinases such as FAK (focal adhesion kinase) and Src kinase family members to phosphorylate substrates such as p130CAS thereby recruiting signaling adaptors such as CRK. These adhesion complexes attach to the actin cytoskeleton. The integrins thus serve to link two networks across the plasma membrane: the extracellular ECM and the intracellular actin filamentous system. Integrin alpha6beta4 is an exception: it links to the keratin intermediate filament system in epithelial cells.

Focal adhesions are large molecular complexes, which are generated following interaction of integrins with ECM, then their clustering. The clusters likely provide sufficient intracellular binding sites to permit the formation of stable signaling complexes on the cytoplasmic side of the cell membrane. So the focal adhesions contain integrin ligand, integrin molecule, and associate plaque proteins. Binding is propelled by changes in free energy.^[12] As previously stated, these complexes connect the extracellular matrix to actin bundles. Cryo-electron tomography reveals that the adhesion contains particles on the cell membrane with diameter of 25 +/- 5 nm and spaced at approximately 45 nm.^[13] Treatment with Rho-kinase inhibitor Y-27632 reduces the size of the particle, and it is extremely mechanosensitive.^[14]

One important function of integrins on cells in tissue culture is their role in cell migration. Cells adhere to a substrate through their integrins. During movement, the cell makes new attachments to the substrate at its front and concurrently releases those at its rear. When released from the substrate, integrin molecules are taken back into the cell by endocytosis; they are transported through the cell to its front by the endocytic cycle where they are added back to the surface. In this way they are cycled for reuse, enabling the cell to make fresh attachments at its leading front. It is not yet clear whether cell migration in tissue culture is an artefact of integrin processing, or whether such integrin dependent cell migration also occurs in living organisms.

Signal transduction

Integrins play an important role in cell signaling.^[15] Connection with ECM molecules can cause a signal to be relayed into the cell through protein kinases that are indirectly and temporarily connected with the intracellular end of the integrin molecule, likely following shape changes directly stimulated by ECM binding.

The signals the cell receives through the integrin can have relation to:

• cell growth,
• cell division,
• cell survival,
• cellular differentiation, and
• apoptosis (programmed cell death).

Vertebrate integrins

The following are some of the integrins found in vertebrates:

Name	Synonyms	Distribution	Ligands
α1β1		Many	Collagens, laminins[16]
α2β1		Many	Collagens, laminins[16]
α4β1	VLA-4[16]	Hematopoietic cells	Fibronectin, VCAM-1[16]
α5β1	fibronectin receptor	widespread	fibronectin[16] and proteinases
α6β1	laminin receptor	widespread	matrix macromolecules laminins
αLβ2	LFA-1[16]	T-lymphocytes	ICAM-1, ICAM-2[16]
αMβ2	Mac-1, CR3[16]	Neutrophils and monocytes	Serum proteins, ICAM-1[16]
αIIbβ3	Vibronectin[17]	Platelets[16]	fibrinogen, fibronectin[16]
αVβ3	vitronectin receptor[18]	activated endothelial cells, melanoma, glioblastoma	vitronectin,[18] fibronectin, fibrinogen, osteopontin, Cyr61
αVβ5		widespread, esp. fibroblasts, epithelial cells	vitronectin and adenovirus
αVβ6		proliferating epithelia, esp. lung and liver	fibronectin; TGFβ1+3
α6β4		Epithelial cells[16]	Laminin[16]

Beta-1 integrins interact with many alpha integrin chains. Gene knockouts of integrins in mice are not always lethal, which proves that during embryonal development, one integrin may substitute its function for another in order to allow survival. Some integrins are on the cell surface in an inactive state, and can be rapidly primed, or put into a state capable of binding their ligands, by cytokines. Integrins can assume several different well-defined shapes or "conformational states". Once primed, the conformational state changes to stimulate ligand binding, which then activates the receptors—also by inducing a shape change—to trigger outside-in signal transduction.

Additional images

• 
  Integrin

References

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2. Xiong JP, Stehle T, Diefenbach B; et al. (2001). "Crystal structure of the extracellular segment of integrin alpha Vbeta3". Science. 294 (5541): 339–45. doi:10.1126/science.1064535. PMC 2885948. PMID 11546839. {{cite journal}}: Explicit use of et al. in: |author= (help); Unknown parameter |month= ignored (help)
3. Humphries M.J. (2000). "Integrin structure". Biochem. Soc. Trans. 28 (4): 311–339. doi:10.1042/0300-5127:0280311. PMID 10961914.
4. Nermut MV, Green NM, Eason P, Yamada SS, Yamada KM (1988). "Electron microscopy and structural model of human fibronectin receptor". EMBO J. 7 (13): 4093–9. PMC 455118. PMID 2977331. {{cite journal}}: Unknown parameter |month= ignored (help)
5. Hynes R (2002). "Integrins: bidirectional, allosteric signaling machines". Cell. 110 (6): 673–87. doi:10.1016/S0092-8674(02)00971-6. PMID 12297042.
6. Xiong JP; Stehle, T; Diefenbach, B; Zhang, R; Dunker, R; Scott, DL; Joachimiak, A; Goodman, SL; Arnaout, MA (2001). "Crystal structure of the extracellular segment of integrin αvβ3". Science. 294 (5541): 339–345. doi:10.1126/science.1064535. PMC 2885948. PMID 11546839.
7. Smith J (2003). "Cilengitide Merck". Curr Opin Investig Drugs. 4 (6): 741–5. PMID 12901235.
8. Calderwood DA (2004). "Talin controls integrin activation". Biochem. Soc. Trans. 32 (Pt3): 434–7. doi:10.1042/BST0320434. PMID 15157154. {{cite journal}}: Unknown parameter |month= ignored (help)
9. Calderwood DA, Zent R, Grant R, Rees DJ, Hynes RO, Ginsberg MH (1999). "The Talin head domain binds to integrin beta subunit cytoplasmic tails and regulates integrin activation". J. Biol. Chem. 274 (40): 28071–4. doi:10.1074/jbc.274.40.28071. PMID 10497155. {{cite journal}}: Unknown parameter |month= ignored (help)
10. Goldmann WH, Bremer A, Häner M, Aebi U, Isenberg G (1994). "Native talin is a dumbbell-shaped homodimer when it interacts with actin". J. Struct. Biol. 112 (1): 3–10. doi:10.1006/jsbi.1994.1002. PMID 8031639.
11. Harburger DS, Bouaouina M, Calderwood DA (2009). "Kindlin-1 and −2 directly bind the C-terminal region of beta integrin cytoplasmic tails and exert integrin-specific activation effects". J. Biol. Chem. 284 (17): 11485–97. doi:10.1074/jbc.M809233200. PMC 2670154. PMID 19240021. {{cite journal}}: Unknown parameter |month= ignored (help)
12. Olberding JE, Thouless MD, Arruda EM, Garikipati K (2010). Buehler, Markus J. (ed.). "The non-equilibrium thermodynamics and kinetics of focal adhesion dynamics". PLoS ONE. 5 (8): e12043. doi:10.1371/journal.pone.0012043. PMC 2923603. PMID 20805876.
13. Patla I, Volberg T, Elad N, Hirschfeld-Warneken V, Grashoff C, Fässler R, Spatz JP, Geiger B, Medalia O (2010). "Dissecting the molecular architecture of integrin adhesion sites by cryo-electron tomography". Nat. Cell Biol. 12 (9): 909–15. doi:10.1038/ncb2095. PMID 20694000. {{cite journal}}: Unknown parameter |month= ignored (help)
14. Gullingsrud J, Sotomayor M. "Mechanosensitive channels". Theoretical and Computational Biophysics Group, Beckman Institute for Advanced Science and Technology: University of Illinois at Urbana-Champaign. {{cite web}}: Cite has empty unknown parameter: |coauthors= (help)
15. Benjamin Lewin (2007). Cells. Jones & Bartlett Learning. pp. 671–. ISBN 978-0-7637-3905-8. Retrieved 26 November 2010.
16. Krieger M, Scott MP, Matsudaira PT, Lodish HF, Darnell JE, Zipursky L, Kaiser C, Berk A (2004). Molecular cell biology (fifth ed.). New York: W.H. Freeman and CO. ISBN 0-7167-4366-3.
17. http://www.vetpathology.org/cgi/reprint/34/1/61.pdf Vet Path01 34:61-73 (1997)
18. Hermann P, Armant M, Brown E, Rubio M, Ishihara H, Ulrich D, Caspary RG, Lindberg FP, Armitage R, Maliszewski C, Delespesse G, Sarfati M (1999). "The vitronectin receptor and its associated CD47 molecule mediates proinflammatory cytokine synthesis in human monocytes by interaction with soluble CD23". J. Cell Biol. 144 (4): 767–75. doi:10.1083/jcb.144.4.767. PMC 2132927. PMID 10037797. {{cite journal}}: Unknown parameter |month= ignored (help)

External links

Media related to Integrins at Wikimedia Commons

• MBInfo - Integrins
• The Integrin Protein
• Talin substrate for calpain – PMAP The Proteolysis Map animation.
• Integrins at the U.S. National Library of Medicine Medical Subject Headings (MeSH)