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cGAS–STING cytosolic DNA sensing pathway

August 25, 2023

The cGAS–STING pathway is a component of the innate immune system that functions to detect the presence of cytosolic DNA and, in response, trigger expression of inflammatory genes that can lead to senescence[1] or to the activation of defense mechanisms. DNA is normally found in the nucleus of the cell. Localization of DNA to the cytosol is associated with tumorigenesis, viral infection, and invasion by some intracellular bacteria.[2] The cGAS – STING pathway acts to detect cytosolic DNA and induce an immune response.

Upon binding DNA, the protein cyclic GMP-AMP Synthase (cGAS) triggers reaction of GTP and ATP to form cyclic GMP-AMP (cGAMP). cGAMP binds to Stimulator of Interferon Genes (STING) which triggers phosphorylation of IRF3 via TBK1. IRF3 can then go to the nucleus to trigger transcription of inflammatory genes. This pathway plays a critical role in mediating immune defense against double-stranded DNA viruses.

The innate immune system relies on germline encoded pattern recognition receptors (PRRs) to recognize distinct pathogen-associated molecular patterns (PAMPs). Upon recognition of a PAMP, PRRs generate signal cascades leading to transcription of genes associated with the immune response. Because all pathogens utilize nucleic acid to propagate, DNA and RNA can be recognized by PRRs to trigger immune activation. In normal cells, DNA is confined to the nucleus or mitochondria. The presence of DNA in the cytosol is indicative of cellular damage or infection and leads to activation of genes associated with the immune response. One way cytosolic DNA is sensed is via the cGAS/STING pathway, specifically by the cyclic-GMP-AMP synthase (cGAS). Upon DNA recognition, cGAS dimerizes and stimulates the formation of cyclic-GMP-AMP (cGAMP). cGAMP then binds directly to stimulator of interferon genes (STING) which triggers phosphorylation/activation of the transcription factor IRF3 via TBK1. IRF3 is able to enter the nucleus to promote transcription of inflammatory genes, such as IFN-β.

Cyclic GMP-AMP synthase (cGAS)

Structure

cGAS is a 522 amino acid protein and a member of the nucleotidyltransferase family. N-terminal residues 1-212 are necessary to bind dsDNA. This region may contain two different DNA binding domains. C-terminal residues 213-522 contain part of the nucleotidyltransferase (NTase) motif and a Mab21 domain and are highly conserved in cGAS from zebrafish to humans. These regions are necessary to form the catalytic pocket for the cGAS substrates: GTP and ATP, and to perform the necessary cyclization reaction.[3][4][5]

Function

cGAS is found at the plasma membrane[6] and is responsible for detecting cytosolic double stranded DNA, normally found in the cell nucleus, in order to stimulate production of IFN-β. cGAS is also found in the nucleus where tight tethering to chromatin prevents its activation by self-DNA.[7] Upon directly binding cytosolic DNA, cGAS forms dimers to catalyze production of 2’3’-cGAMP from ATP and GTP. cGAMP then acts a second messenger, binding to STING, to trigger activation of the transcription factor IRF3. IRF3 leads to transcription of type-1 IFN-β. cGAS is unable to produce 2’3’-cGAMP in the presence of RNA.

Discovery

Prior to the discovery of cGAS, it was known that interferon beta was produced in the presence of cytosolic dsDNA and that STING-deficient cells were unable to produce interferon in the presence of dsDNA. Through biochemical fractionation of cell extracts and quantitative mass spectrometry, Sun, et al.[8] identified cGAS as the DNA-sensing protein able to trigger interferon beta by synthesizing the second messenger, 2’3’-cGAMP. This activity is dependent on cytosolic DNA.

Enzymatic activity

cGAS catalyzes formation of cGAMP in the presence of dsDNA. cGAS directly binds dsDNA via positively charged amino acid residues interacting with the negatively charged DNA phosphate backbone. Mutations in the positively charged residues completely abrogate DNA binding and subsequent interferon production through STING. Upon binding dsDNA, cGAS dimerizes and undergoes conformational changes that open up a catalytic nucleotide binding pocket, allowing GTP and ATP to enter. Here they are stabilized through base stacking, hydrogen bonds, and divalent cations in order to catalyze phosphodiester bond formation to produce the cyclic dinucleotide cGAMP.

Cyclic GMP-AMP (cGAMP)

Main article: Cyclic GMP-AMP synthase

Structure

Cyclic GMP-AMP (cGAMP) is a cyclic dinucleotide (CDN) and the first to be found in metazoans. Other CDNs (c-di-GMP and c-di-AMP) are commonly found in bacteria, archaea, and protozoa. As the name suggests, cGAMP is cyclic molecule composed of one Adenine monophosphate (AMP) and one Guanine monophosphate (GMP) connected by two phosphodiester bonds. However, cGAMP differs from other CDNs in that it contains a unique phosphodiester bonds between the 2’ OH of GMP and the 5’ phosphate of AMP.[9] The other bond is between the 3’ OH of AMP and the 5’ phosphate of GMP. The unique 2’-5’ phosphodiester bond may be advantageous because it is less susceptible to degradation caused by 3’-5’ phosphodiesterases. Other advantages of the unique 2’-5’ linkage may be that cGAMP is able to bind multiple allelic variants of STING found in the human population, while other CDNs, composed of only 3’-5’ linkages, are not.

 
cGAS bound to dsDNA. Adapted from PDB 4O6A.[10]

Discovery

cGAMP was discovered by Zhijian "James" Chen and colleagues[11] by collecting cytoplasmic extracts from cells transfected with different types of DNA. Cellular extracts were assayed for STING activation by detecting activated IRF3 dimers. Using affinity purification chromatography, the STING activating substance was purified and mass spectrometry was used to identify the substance as cyclic-GMP-AMP (cGAMP).

Chemically synthesized cGAMP was shown to trigger IRF3 activation and IFN-β production. cGAMP was found to be much more potent than other cyclic di-nucleotides (c-di-GMP and c-di-AMP). cGAMP was shown to definitively bind STING by using radiolabeled cGAMP cross-linked to STING. Adding in unlabeled cGAMP, c-di-GMP, or c-di-AMP was found to compete with radio-labeled cGAMP, suggesting that CDN binding sites overlap. It was later shown that cGAMP has a unique 2’-5’ phosphodiester bond, which differs from conventional 3’-5’ linked CDNs and that this bond may explain some of the unique signaling properties of cGAMP.[9]

Stimulator of Interferon Genes (STING)

Main article: Stimulator of Interferon Genes

STING is an endoplasmic reticulum resident protein and has been shown to directly bind to a variety of different cyclic-di-nucleotides.[9]

Expression

STING is expressed broadly in numerous tissue types, of both immune and non-immune origin.[12] STING was identified in murine embryonic fibroblasts, and is required for the type 1 interferon response in both immune and non-immune cells.[13]

Structure

STING is a 378 amino acid protein. Its N-terminal region (residues 1-154) contains four trans-membrane domains. Its C-terminal domain contains the dimerization domain, the cyclic dinucleotide interaction domain, as well as a domain responsible for interacting and activating TBK1. Upon binding of 2’-3’ cGAMP, STING undergoes a significant conformational change (approximately 20 Angstrom inward rotation) that encloses cGAMP.

 
STING bound to cGAMP. While STING exists as a homodimer, only one subunit is shown to highlight the interaction of side chain residues with cGAMP. Adapted from PDB 4KSY [14]

Function

Upon binding of 2’-3’ cGAMP (and other bacterial CDNs), STING activates TBK1 to phosphorylate downstream transcription factors IRF3, which induces the type 1 IFN response, and STAT6, which induces chemokines such as CCL2 and CCL20 independently of IRF3.[15] STING is also thought to activate the NF-κB transcription factor through the activity of the IκB kinase (IKK), though the mechanism of NF-κB activation downstream of STING remains to be determined. The signaling pathways activated by STING combine to induce an innate immune response to cells with ectopic DNA in the cytosol. Loss of STING activity inhibits the ability of mouse embryonic fibroblasts to fight against infection by certain viruses, and more generally, is required for the type 1 IFN response to introduced cytosolic DNA.[13]

STING’s general role as an adapter molecule in the cytosolic DNA-type 1 IFN response across cell types has been suggested to function through dendritic cells (DCs). DCs link the innate immune system with the adaptive immune system through phagocytosis and MHC presentation of foreign antigen. The type 1 IFN response initiated by DCs, perhaps through recognition of phagocytosed DNA,[16] has an important co-stimulatory effect. This has recently led to speculation that 2’-3’ cGAMP could be used as a more efficient and direct adjuvant than DNA to induce immune responses.

Allelic Variation

Naturally occurring variations in human STING (hSTING) have been found at amino acid position 232 (R232 and H232). H232 variants have diminished type 1 IFN responses[17] and mutation at this position to alanine abrogates the response to bacterial CDNs. Substitutions enhancing ligand binding were also found. G230A substitutions were shown to increase hSTING signaling upon c-di-GMP binding. This residue is found on the lid of the binding pocket, possibly increasing c-di-GMP binding ability.[18]

Biological Importance of the cGAS-STING pathway

Role in viral response

The cGAS-cGAMP-STING pathway is able to generate interferon beta in response to cytosolic DNA. It was shown that DNA viruses, such as HSV-1, are able to trigger cGAMP production and subsequent activation of interferon beta via STING . RNA viruses, such as VSV or Sendai virus, are unable to trigger interferon via cGAS-STING. cGAS or STING defective mice are unable to produce interferon in response to HSV-1 infection which eventually leads to death, while mice with normal cGAS and STING function are able to recover.

Retroviruses, such as HIV-1, were also shown to activate IFN via the cGAS/STING pathway. In these studies, inhibitors of retroviral reverse transcription abrogated IFN production, suggesting that it is the viral cDNA which is activating cGAS.[19]

Role in tumor surveillance

The cGAS/STING pathway also has a role in tumor surveillance. In response to cellular stress, such as DNA damage, cells will upregulate NKG2D ligands so that they may be recognized and destroyed by Natural Killer (NK) and T cells. In many tumor cells, the DNA damage response is constitutively active, leading to the accumulation of cytoplasmic DNA. This activates the cGAS/STING pathway leading to activation of IRF3. It was shown in lymphoma cells that the NKG2D ligand, Rae1, was upregulated in a STING/IRF3 dependent manner. Transfection of DNA into these cells also triggered Rae1 expression that was dependent on STING. In this model, the transcription factor IRF3, via cGAS/STING, upregulates stress-induced ligands, such as Rae1, in tumor cells, so as to aid in NK-mediated tumor clearance. [20] Moreover, activation of the STING pathway in bone marrow macrophages has been shown to inhibit the growth of acute myeloid leukaemia cells in mice models. [21]

Role in autoimmune disease

Cytoplasmic DNA, due to viral infection, can lead to activation of interferon beta to help clear the infection. However, chronic activation of STING, due to host DNA in the cytosol, can also activate the cGAS/STING pathway, leading to autoimmune disorders. An example of this occurs in Aicardi–Goutières syndrome (AGS). Mutations in the 3’ repair exonuclease, TREX1, cause endogenous retroelements to accumulate in the cytosol, which can lead to cGAS/STING activation, resulting in IFN production. Excessive IFN production leads to an over-active immune system, resulting in AGS and other immune disorders. In mice, it was found that autoimmune symptoms associated with TREX1 deficiency were relieved by cGAS, STING, or IRF3 knockout, implying the importance of aberrant DNA sensing in autoimmune disorders.[19]

Role in cellular senescence

It has been shown that the depletion of cGAS and STING in mouse embryonic fibroblasts and in primary human fibroblasts prevents senescence and SASP (senescence-associated secretory phenotype) establishment.[22][1]

Therapeutic role

Potential vaccine adjuvant

DNA has been shown to be a potent adjuvant to boost the immune response to antigens encoded by vaccines. cGAMP, through IRF3 activation of STING, stimulates transcription of interferon. This makes cGAMP a potential vaccine adjuvant capable of boosting inflammatory responses.[9] Studies have shown that vaccines encoded with the chicken antigen, ovalbumin (OVA), in conjunction with cGAMP, were able to activate antigen-specific T and B cells in a STING-dependent manner in vivo. When stimulated with OVA peptide, the T cells from mice vaccinated with OVA + cGAMP were shown to have elevated IFN-g and IL-2 when compared to animals receiving only OVA.[23] Furthermore, the enhanced stability of cGAMP, due to the unique 2’-5’ phosphodiester bond, may make it a preferred adjuvant to DNA for in vivo applications.

References

  1. ^ a b Yang H, Wang H, Ren J, Chen Q, Chen ZJ (June 2017). "cGAS is essential for cellular senescence". Proceedings of the National Academy of Sciences of the United States of America. 114 (23): E4612–E4620. Bibcode:2017PNAS..114E4612Y. doi:10.1073/pnas.1705499114. PMC 5468617. PMID 28533362.
  2. ^ Watson RO, Bell SL, MacDuff DA, Kimmey JM, Diner EJ, Olivas J, et al. (June 2015). "The Cytosolic Sensor cGAS Detects Mycobacterium tuberculosis DNA to Induce Type I Interferons and Activate Autophagy". Cell Host & Microbe. 17 (6): 811–819. doi:10.1016/j.chom.2015.05.004. PMC 4466081. PMID 26048136.
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  9. ^ a b c d Diner EJ, Burdette DL, Wilson SC, Monroe KM, Kellenberger CA, Hyodo M, et al. (May 2013). "The innate immune DNA sensor cGAS produces a noncanonical cyclic dinucleotide that activates human STING". Cell Reports. 3 (5): 1355–61. doi:10.1016/j.celrep.2013.05.009. PMC 3706192. PMID 23707065.
  10. ^ PDB: 4O6A
  11. ^ Wu J, Sun L, Chen X, Du F, Shi H, Chen C, Chen ZJ (February 2013). "Cyclic GMP-AMP is an endogenous second messenger in innate immune signaling by cytosolic DNA". Science. 339 (6121): 826–30. Bibcode:2013Sci...339..826W. doi:10.1126/science.1229963. PMC 3855410. PMID 23258412.
  12. ^ "TMEM173 Expression". Gene Cards.
  13. ^ a b Ishikawa H, Ma Z, Barber GN (October 2009). "STING regulates intracellular DNA-mediated, type I interferon-dependent innate immunity". Nature. 461 (7265): 788–92. Bibcode:2009Natur.461..788I. doi:10.1038/nature08476. PMC 4664154. PMID 19776740.
  14. ^ PDB: 4KSY
  15. ^ Burdette DL, Monroe KM, Sotelo-Troha K, Iwig JS, Eckert B, Hyodo M, et al. (September 2011). "STING is a direct innate immune sensor of cyclic di-GMP". Nature. 478 (7370): 515–8. Bibcode:2011Natur.478..515B. doi:10.1038/nature10429. PMC 3203314. PMID 21947006.
  16. ^ Woo SR, Fuertes MB, Corrales L, Spranger S, Furdyna MJ, Leung MY, et al. (November 2014). "STING-dependent cytosolic DNA sensing mediates innate immune recognition of immunogenic tumors". Immunity. 41 (5): 830–42. doi:10.1016/j.immuni.2014.10.017. PMC 4384884. PMID 25517615.
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  18. ^ Yi G, Brendel VP, Shu C, Li P, Palanathan S, Cheng Kao C (2013). "Single nucleotide polymorphisms of human STING can affect innate immune response to cyclic dinucleotides". PLOS ONE. 8 (10): e77846. Bibcode:2013PLoSO...877846Y. doi:10.1371/journal.pone.0077846. PMC 3804601. PMID 24204993.
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  20. ^ Lam AR, Bert NL, Ho SS, Shen YJ, Tang LF, Xiong GM, et al. (April 2014). "RAE1 ligands for the NKG2D receptor are regulated by STING-dependent DNA sensor pathways in lymphoma". Cancer Research. 74 (8): 2193–2203. doi:10.1158/0008-5472.CAN-13-1703. PMC 4229084. PMID 24590060.
  21. ^ Moore, Jamie A.; Mistry, Jayna J.; Hellmich, Charlotte; Horton, Rebecca H.; Wojtowicz, Edyta E.; Jibril, Aisha; Jefferson, Matthew; Wileman, Thomas; Beraza, Naiara; Bowles, Kristian M.; Rushworth, Stuart A. (2022-01-06). "LC3-associated phagocytosis in bone marrow macrophages suppresses acute myeloid leukemia progression through STING activation". The Journal of Clinical Investigation. 132 (5). doi:10.1172/JCI153157. ISSN 0021-9738. PMC 8884913. PMID 34990402.
  22. ^ Glück S, Guey B, Gulen MF, Wolter K, Kang TW, Schmacke NA, et al. (September 2017). "Innate immune sensing of cytosolic chromatin fragments through cGAS promotes senescence". Nature Cell Biology. 19 (9): 1061–1070. doi:10.1038/ncb3586. PMC 5826565. PMID 28759028.
  23. ^ Li XD, Wu J, Gao D, Wang H, Sun L, Chen ZJ (September 2013). "Pivotal roles of cGAS-cGAMP signaling in antiviral defense and immune adjuvant effects". Science. 341 (6152): 1390–4. Bibcode:2013Sci...341.1390L. doi:10.1126/science.1244040. PMC 3863637. PMID 23989956.

August 25, 2023
cgas, sting, cytosolic, sensing, pathway, cgas, sting, pathway, component, innate, immune, system, that, functions, detect, presence, cytosolic, response, trigger, expression, inflammatory, genes, that, lead, senescence, activation, defense, mechanisms, normal. The cGAS STING pathway is a component of the innate immune system that functions to detect the presence of cytosolic DNA and in response trigger expression of inflammatory genes that can lead to senescence 1 or to the activation of defense mechanisms DNA is normally found in the nucleus of the cell Localization of DNA to the cytosol is associated with tumorigenesis viral infection and invasion by some intracellular bacteria 2 The cGAS STING pathway acts to detect cytosolic DNA and induce an immune response Upon binding DNA the protein cyclic GMP AMP Synthase cGAS triggers reaction of GTP and ATP to form cyclic GMP AMP cGAMP cGAMP binds to Stimulator of Interferon Genes STING which triggers phosphorylation of IRF3 via TBK1 IRF3 can then go to the nucleus to trigger transcription of inflammatory genes This pathway plays a critical role in mediating immune defense against double stranded DNA viruses The innate immune system relies on germline encoded pattern recognition receptors PRRs to recognize distinct pathogen associated molecular patterns PAMPs Upon recognition of a PAMP PRRs generate signal cascades leading to transcription of genes associated with the immune response Because all pathogens utilize nucleic acid to propagate DNA and RNA can be recognized by PRRs to trigger immune activation In normal cells DNA is confined to the nucleus or mitochondria The presence of DNA in the cytosol is indicative of cellular damage or infection and leads to activation of genes associated with the immune response One way cytosolic DNA is sensed is via the cGAS STING pathway specifically by the cyclic GMP AMP synthase cGAS Upon DNA recognition cGAS dimerizes and stimulates the formation of cyclic GMP AMP cGAMP cGAMP then binds directly to stimulator of interferon genes STING which triggers phosphorylation activation of the transcription factor IRF3 via TBK1 IRF3 is able to enter the nucleus to promote transcription of inflammatory genes such as IFN b Contents 1 Cyclic GMP AMP synthase cGAS 1 1 Structure 1 2 Function 1 3 Discovery 1 4 Enzymatic activity 2 Cyclic GMP AMP cGAMP 2 1 Structure 2 2 Discovery 3 Stimulator of Interferon Genes STING 3 1 Expression 3 2 Structure 3 3 Function 3 4 Allelic Variation 4 Biological Importance of the cGAS STING pathway 4 1 Role in viral response 4 2 Role in tumor surveillance 4 3 Role in autoimmune disease 4 4 Role in cellular senescence 4 5 Therapeutic role 4 5 1 Potential vaccine adjuvant 5 ReferencesCyclic GMP AMP synthase cGAS EditStructure Edit cGAS is a 522 amino acid protein and a member of the nucleotidyltransferase family N terminal residues 1 212 are necessary to bind dsDNA This region may contain two different DNA binding domains C terminal residues 213 522 contain part of the nucleotidyltransferase NTase motif and a Mab21 domain and are highly conserved in cGAS from zebrafish to humans These regions are necessary to form the catalytic pocket for the cGAS substrates GTP and ATP and to perform the necessary cyclization reaction 3 4 5 Function Edit cGAS is found at the plasma membrane 6 and is responsible for detecting cytosolic double stranded DNA normally found in the cell nucleus in order to stimulate production of IFN b cGAS is also found in the nucleus where tight tethering to chromatin prevents its activation by self DNA 7 Upon directly binding cytosolic DNA cGAS forms dimers to catalyze production of 2 3 cGAMP from ATP and GTP cGAMP then acts a second messenger binding to STING to trigger activation of the transcription factor IRF3 IRF3 leads to transcription of type 1 IFN b cGAS is unable to produce 2 3 cGAMP in the presence of RNA Discovery Edit Prior to the discovery of cGAS it was known that interferon beta was produced in the presence of cytosolic dsDNA and that STING deficient cells were unable to produce interferon in the presence of dsDNA Through biochemical fractionation of cell extracts and quantitative mass spectrometry Sun et al 8 identified cGAS as the DNA sensing protein able to trigger interferon beta by synthesizing the second messenger 2 3 cGAMP This activity is dependent on cytosolic DNA Enzymatic activity Edit cGAS catalyzes formation of cGAMP in the presence of dsDNA cGAS directly binds dsDNA via positively charged amino acid residues interacting with the negatively charged DNA phosphate backbone Mutations in the positively charged residues completely abrogate DNA binding and subsequent interferon production through STING Upon binding dsDNA cGAS dimerizes and undergoes conformational changes that open up a catalytic nucleotide binding pocket allowing GTP and ATP to enter Here they are stabilized through base stacking hydrogen bonds and divalent cations in order to catalyze phosphodiester bond formation to produce the cyclic dinucleotide cGAMP Cyclic GMP AMP cGAMP EditMain article Cyclic GMP AMP synthase Structure Edit Cyclic GMP AMP cGAMP is a cyclic dinucleotide CDN and the first to be found in metazoans Other CDNs c di GMP and c di AMP are commonly found in bacteria archaea and protozoa As the name suggests cGAMP is cyclic molecule composed of one Adenine monophosphate AMP and one Guanine monophosphate GMP connected by two phosphodiester bonds However cGAMP differs from other CDNs in that it contains a unique phosphodiester bonds between the 2 OH of GMP and the 5 phosphate of AMP 9 The other bond is between the 3 OH of AMP and the 5 phosphate of GMP The unique 2 5 phosphodiester bond may be advantageous because it is less susceptible to degradation caused by 3 5 phosphodiesterases Other advantages of the unique 2 5 linkage may be that cGAMP is able to bind multiple allelic variants of STING found in the human population while other CDNs composed of only 3 5 linkages are not cGAS bound to dsDNA Adapted from PDB 4O6A 10 Discovery Edit cGAMP was discovered by Zhijian James Chen and colleagues 11 by collecting cytoplasmic extracts from cells transfected with different types of DNA Cellular extracts were assayed for STING activation by detecting activated IRF3 dimers Using affinity purification chromatography the STING activating substance was purified and mass spectrometry was used to identify the substance as cyclic GMP AMP cGAMP Chemically synthesized cGAMP was shown to trigger IRF3 activation and IFN b production cGAMP was found to be much more potent than other cyclic di nucleotides c di GMP and c di AMP cGAMP was shown to definitively bind STING by using radiolabeled cGAMP cross linked to STING Adding in unlabeled cGAMP c di GMP or c di AMP was found to compete with radio labeled cGAMP suggesting that CDN binding sites overlap It was later shown that cGAMP has a unique 2 5 phosphodiester bond which differs from conventional 3 5 linked CDNs and that this bond may explain some of the unique signaling properties of cGAMP 9 Stimulator of Interferon Genes STING EditMain article Stimulator of Interferon Genes STING is an endoplasmic reticulum resident protein and has been shown to directly bind to a variety of different cyclic di nucleotides 9 Expression Edit STING is expressed broadly in numerous tissue types of both immune and non immune origin 12 STING was identified in murine embryonic fibroblasts and is required for the type 1 interferon response in both immune and non immune cells 13 Structure Edit STING is a 378 amino acid protein Its N terminal region residues 1 154 contains four trans membrane domains Its C terminal domain contains the dimerization domain the cyclic dinucleotide interaction domain as well as a domain responsible for interacting and activating TBK1 Upon binding of 2 3 cGAMP STING undergoes a significant conformational change approximately 20 Angstrom inward rotation that encloses cGAMP STING bound to cGAMP While STING exists as a homodimer only one subunit is shown to highlight the interaction of side chain residues with cGAMP Adapted from PDB 4KSY 14 Function Edit Upon binding of 2 3 cGAMP and other bacterial CDNs STING activates TBK1 to phosphorylate downstream transcription factors IRF3 which induces the type 1 IFN response and STAT6 which induces chemokines such as CCL2 and CCL20 independently of IRF3 15 STING is also thought to activate the NF kB transcription factor through the activity of the IkB kinase IKK though the mechanism of NF kB activation downstream of STING remains to be determined The signaling pathways activated by STING combine to induce an innate immune response to cells with ectopic DNA in the cytosol Loss of STING activity inhibits the ability of mouse embryonic fibroblasts to fight against infection by certain viruses and more generally is required for the type 1 IFN response to introduced cytosolic DNA 13 STING s general role as an adapter molecule in the cytosolic DNA type 1 IFN response across cell types has been suggested to function through dendritic cells DCs DCs link the innate immune system with the adaptive immune system through phagocytosis and MHC presentation of foreign antigen The type 1 IFN response initiated by DCs perhaps through recognition of phagocytosed DNA 16 has an important co stimulatory effect This has recently led to speculation that 2 3 cGAMP could be used as a more efficient and direct adjuvant than DNA to induce immune responses Allelic Variation Edit Naturally occurring variations in human STING hSTING have been found at amino acid position 232 R232 and H232 H232 variants have diminished type 1 IFN responses 17 and mutation at this position to alanine abrogates the response to bacterial CDNs Substitutions enhancing ligand binding were also found G230A substitutions were shown to increase hSTING signaling upon c di GMP binding This residue is found on the lid of the binding pocket possibly increasing c di GMP binding ability 18 Biological Importance of the cGAS STING pathway EditRole in viral response Edit The cGAS cGAMP STING pathway is able to generate interferon beta in response to cytosolic DNA It was shown that DNA viruses such as HSV 1 are able to trigger cGAMP production and subsequent activation of interferon beta via STING RNA viruses such as VSV or Sendai virus are unable to trigger interferon via cGAS STING cGAS or STING defective mice are unable to produce interferon in response to HSV 1 infection which eventually leads to death while mice with normal cGAS and STING function are able to recover Retroviruses such as HIV 1 were also shown to activate IFN via the cGAS STING pathway In these studies inhibitors of retroviral reverse transcription abrogated IFN production suggesting that it is the viral cDNA which is activating cGAS 19 Role in tumor surveillance Edit The cGAS STING pathway also has a role in tumor surveillance In response to cellular stress such as DNA damage cells will upregulate NKG2D ligands so that they may be recognized and destroyed by Natural Killer NK and T cells In many tumor cells the DNA damage response is constitutively active leading to the accumulation of cytoplasmic DNA This activates the cGAS STING pathway leading to activation of IRF3 It was shown in lymphoma cells that the NKG2D ligand Rae1 was upregulated in a STING IRF3 dependent manner Transfection of DNA into these cells also triggered Rae1 expression that was dependent on STING In this model the transcription factor IRF3 via cGAS STING upregulates stress induced ligands such as Rae1 in tumor cells so as to aid in NK mediated tumor clearance 20 Moreover activation of the STING pathway in bone marrow macrophages has been shown to inhibit the growth of acute myeloid leukaemia cells in mice models 21 Role in autoimmune disease Edit Cytoplasmic DNA due to viral infection can lead to activation of interferon beta to help clear the infection However chronic activation of STING due to host DNA in the cytosol can also activate the cGAS STING pathway leading to autoimmune disorders An example of this occurs in Aicardi Goutieres syndrome AGS Mutations in the 3 repair exonuclease TREX1 cause endogenous retroelements to accumulate in the cytosol which can lead to cGAS STING activation resulting in IFN production Excessive IFN production leads to an over active immune system resulting in AGS and other immune disorders In mice it was found that autoimmune symptoms associated with TREX1 deficiency were relieved by cGAS STING or IRF3 knockout implying the importance of aberrant DNA sensing in autoimmune disorders 19 Role in cellular senescence Edit It has been shown that the depletion of cGAS and STING in mouse embryonic fibroblasts and in primary human fibroblasts prevents senescence and SASP senescence associated secretory phenotype establishment 22 1 Therapeutic role Edit Potential vaccine adjuvant Edit DNA has been shown to be a potent adjuvant to boost the immune response to antigens encoded by vaccines cGAMP through IRF3 activation of STING stimulates transcription of interferon This makes cGAMP a potential vaccine adjuvant capable of boosting inflammatory responses 9 Studies have shown that vaccines encoded with the chicken antigen ovalbumin OVA in conjunction with cGAMP were able to activate antigen specific T and B cells in a STING dependent manner in vivo When stimulated with OVA peptide the T cells from mice vaccinated with OVA cGAMP were shown to have elevated IFN g and IL 2 when compared to animals receiving only OVA 23 Furthermore the enhanced stability of cGAMP due to the unique 2 5 phosphodiester bond may make it a preferred adjuvant to DNA for in vivo applications References Edit a b Yang H Wang H Ren J Chen Q Chen ZJ June 2017 cGAS is essential for cellular senescence Proceedings of the National Academy of Sciences of the United States of America 114 23 E4612 E4620 Bibcode 2017PNAS 114E4612Y doi 10 1073 pnas 1705499114 PMC 5468617 PMID 28533362 Watson RO Bell SL MacDuff DA Kimmey JM Diner EJ Olivas J et al June 2015 The Cytosolic Sensor cGAS Detects Mycobacterium tuberculosis DNA to Induce Type I Interferons and Activate Autophagy Cell Host amp Microbe 17 6 811 819 doi 10 1016 j chom 2015 05 004 PMC 4466081 PMID 26048136 Ablasser A Schmid Burgk JL Hemmerling I Horvath GL Schmidt T Latz E Hornung V November 2013 Cell intrinsic immunity spreads to bystander cells via the intercellular transfer of cGAMP Nature 503 7477 530 4 Bibcode 2013Natur 503 530A doi 10 1038 nature12640 PMC 4142317 PMID 24077100 Li Y Lu J Han Y Fan X Ding SW October 2013 RNA interference functions as an antiviral immunity mechanism in mammals Science 342 6155 231 4 Bibcode 2013Sci 342 231L doi 10 1126 science 1241911 PMC 3875315 PMID 24115437 Kranzusch PJ Vance RE December 2013 cGAS dimerization entangles DNA recognition Immunity 39 6 992 4 doi 10 1016 j immuni 2013 11 012 PMID 24332024 Barnett KC Coronas Serna JM Zhou W Ernandes MJ Cao A Kranzusch PJ Kagan JC March 2019 Phosphoinositide Interactions Position cGAS at the Plasma Membrane to Ensure Efficient Distinction between Self and Viral DNA Cell 176 6 1432 1446 e11 doi 10 1016 j cell 2019 01 049 PMC 6697112 PMID 30827685 Volkman H E Cambier S Gray E E Stetson D B 2019 Tight nuclear tethering of cGAS is essential for preventing autoreactivity eLife 8 doi 10 7554 eLife 47491 PMC 6927687 PMID 31808743 Sun L Wu J Du F Chen X Chen ZJ February 2013 Cyclic GMP AMP synthase is a cytosolic DNA sensor that activates the type I interferon pathway Science 339 6121 786 91 Bibcode 2013Sci 339 786S doi 10 1126 science 1232458 PMC 3863629 PMID 23258413 a b c d Diner EJ Burdette DL Wilson SC Monroe KM Kellenberger CA Hyodo M et al May 2013 The innate immune DNA sensor cGAS produces a noncanonical cyclic dinucleotide that activates human STING Cell Reports 3 5 1355 61 doi 10 1016 j celrep 2013 05 009 PMC 3706192 PMID 23707065 PDB 4O6A Wu J Sun L Chen X Du F Shi H Chen C Chen ZJ February 2013 Cyclic GMP AMP is an endogenous second messenger in innate immune signaling by cytosolic DNA Science 339 6121 826 30 Bibcode 2013Sci 339 826W doi 10 1126 science 1229963 PMC 3855410 PMID 23258412 TMEM173 Expression Gene Cards a b Ishikawa H Ma Z Barber GN October 2009 STING regulates intracellular DNA mediated type I interferon dependent innate immunity Nature 461 7265 788 92 Bibcode 2009Natur 461 788I doi 10 1038 nature08476 PMC 4664154 PMID 19776740 PDB 4KSY Burdette DL Monroe KM Sotelo Troha K Iwig JS Eckert B Hyodo M et al September 2011 STING is a direct innate immune sensor of cyclic di GMP Nature 478 7370 515 8 Bibcode 2011Natur 478 515B doi 10 1038 nature10429 PMC 3203314 PMID 21947006 Woo SR Fuertes MB Corrales L Spranger S Furdyna MJ Leung MY et al November 2014 STING dependent cytosolic DNA sensing mediates innate immune recognition of immunogenic tumors Immunity 41 5 830 42 doi 10 1016 j immuni 2014 10 017 PMC 4384884 PMID 25517615 Cai X Chiu YH Chen ZJ April 2014 The cGAS cGAMP STING pathway of cytosolic DNA sensing and signaling Molecular Cell 54 2 289 96 doi 10 1016 j molcel 2014 03 040 PMID 24766893 Yi G Brendel VP Shu C Li P Palanathan S Cheng Kao C 2013 Single nucleotide polymorphisms of human STING can affect innate immune response to cyclic dinucleotides PLOS ONE 8 10 e77846 Bibcode 2013PLoSO 877846Y doi 10 1371 journal pone 0077846 PMC 3804601 PMID 24204993 a b Gao D Wu J Wu YT Du F Aroh C Yan N et al August 2013 Cyclic GMP AMP synthase is an innate immune sensor of HIV and other retroviruses Science 341 6148 903 6 Bibcode 2013Sci 341 903G doi 10 1126 science 1240933 PMC 3860819 PMID 23929945 Lam AR Bert NL Ho SS Shen YJ Tang LF Xiong GM et al April 2014 RAE1 ligands for the NKG2D receptor are regulated by STING dependent DNA sensor pathways in lymphoma Cancer Research 74 8 2193 2203 doi 10 1158 0008 5472 CAN 13 1703 PMC 4229084 PMID 24590060 Moore Jamie A Mistry Jayna J Hellmich Charlotte Horton Rebecca H Wojtowicz Edyta E Jibril Aisha Jefferson Matthew Wileman Thomas Beraza Naiara Bowles Kristian M Rushworth Stuart A 2022 01 06 LC3 associated phagocytosis in bone marrow macrophages suppresses acute myeloid leukemia progression through STING activation The Journal of Clinical Investigation 132 5 doi 10 1172 JCI153157 ISSN 0021 9738 PMC 8884913 PMID 34990402 Gluck S Guey B Gulen MF Wolter K Kang TW Schmacke NA et al September 2017 Innate immune sensing of cytosolic chromatin fragments through cGAS promotes senescence Nature Cell Biology 19 9 1061 1070 doi 10 1038 ncb3586 PMC 5826565 PMID 28759028 Li XD Wu J Gao D Wang H Sun L Chen ZJ September 2013 Pivotal roles of cGAS cGAMP signaling in antiviral defense and immune adjuvant effects Science 341 6152 1390 4 Bibcode 2013Sci 341 1390L doi 10 1126 science 1244040 PMC 3863637 PMID 23989956 Retrieved from https en wikipedia org w index php title CGAS STING cytosolic DNA sensing pathway amp oldid 1168515369, wikipedia, wiki, book, books, library,

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