Sulfolobus solfataricus: Difference between revisions
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''S. solfataricus'' is able to oxidizing sulfur in according to metabolic strategy, one of the products of these reactions is H+ and, consequentially, it’s results in a slowly acidification of surrounding area. Soil acidification increase in place where there are emmissions of pollutants from industrial activity, and this process reduce the number of heterotrophic bacterial involved to decomposition, which are foundamental to recycling organic matter and ultimately to fertilizing soil.<ref>{{cite journal | vauthors = Bryant RD, Gordy EA, Laishley EJ |title=Effect of soil acidification on the soil microflora|journal=Water, Air, and Soil Pollution |volume=11 |issue=4 |pages=437 |doi=10.1007/BF00283435 |year=1979 |bibcode=1979WASP...11..437B }}</ref> |
''S. solfataricus'' is able to oxidizing sulfur in according to metabolic strategy, one of the products of these reactions is H+ and, consequentially, it’s results in a slowly acidification of surrounding area. Soil acidification increase in place where there are emmissions of pollutants from industrial activity, and this process reduce the number of heterotrophic bacterial involved to decomposition, which are foundamental to recycling organic matter and ultimately to fertilizing soil.<ref>{{cite journal | vauthors = Bryant RD, Gordy EA, Laishley EJ |title=Effect of soil acidification on the soil microflora|journal=Water, Air, and Soil Pollution |volume=11 |issue=4 |pages=437 |doi=10.1007/BF00283435 |year=1979 |bibcode=1979WASP...11..437B }}</ref> |
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== <big>Biotechnologie</big> == |
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== Untapping the resource ''Sulfolobus'' == |
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Today, in many fields of application, we are interested in using ''Sulfolobus sulfataricus'' as a source of thermal stability enzymes for research and diagnostics, as well as in the food, textile and cleanning industries, and the pulp and paper industry.Furthermore, this enzyme is overloaded due to its catalytic diversity, high pH and temperature stability, increased to organic solvents and resistance to proteolysis.<ref>{{Cite journal|last=Stepankova|first=Veronika|date=October 14, 2013|title=Strategies for Stabilization of Enzymes in Organic Solvents|url=https://doi.org/10.1021/cs400684x|journal=ACS Catalysis|volume=3|pages=2823-2836|via=}}</ref><ref>{{Cite journal|last=DANIEL|first=R. M.|date=1982|title=A correlation between protein thermostability and resistance to proteolysis|url=https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1153914/pdf/biochemj00364-0270.pdf|journal=Biochem. J.|volume=207|pages=641-644|via=}}</ref> |
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At present, tetraester lipids, membrane vesicles with antimicrobial properties, trehalose components, and new β-galactooligosaccharides are coming increasingly important.<ref name=":02">{{Cite journal|last=Quehenberger|first=Julian|date=2017|title=Sulfolobus – A Potential Key Organism in Future Biotechnology|url=https://dx.doi.org/10.3389%2Ffmicb.2017.02474|journal=Front Microbiol.|volume=8:2474|pages=|via=Frontiers Media SA}}</ref> |
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=== [[Beta-galactosidase|β-galactosidase]] === |
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The thermostable enzyme [[Beta-galactosidase|β-galactosidase]] isolated from the extreme thermophile archaebacterial ''[[Sulfolobus solfataricus]] , strain MT-4.'' |
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This enzyme utilized on many industrial process of lactose containing fluids by purifying and characterizing for their physicochemical properties.<ref>{{Cite journal|last=M. PISANI|first=Francesca|date=1990|title=Thermostable P-galactosidase from the archaebacterium Sulfolobus solfataricus|url=https://febs.onlinelibrary.wiley.com/doi/epdf/10.1111/j.1432-1033.1990.tb15308.x|journal=Eur. J. Biochem.|volume=187|pages=321 -328|via=}}</ref> |
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=== [[Protease|Proteases]] === |
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The industry are interested in stable proteases as well as in many different sulfolobus proteases that have been studied. <ref>{{Cite book|url=https://doi.org/10.1016/0304-4165(90)90005-H|title=Isolation and characterization of an intracellular aminopeptidase from the extreme thermophilic archaebacterium Sulfolobus solfataricus|last=Hanner|first=Markus|publisher=Elsevier B.V.|year=1990|isbn=0117536121|location=|pages=148–153}}</ref> |
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An active [[aminopeptidase]] associated with the [[Chaperonin ATPase|chaperonin]] of Solfobulus solfataricus MT4 was described''.''<ref>{{Cite journal|last=Condo|first=Ivano|last2=Ruggero|first2=Davide|date=1998|title=A novel aminopeptidase associated with the 60 kDa chaperonin in the thermophilic archaeon Sulfolobus solfataricus. Mol. Microbiol.|url=https://doi.org/10.1046/j.1365-2958.1998.00971.x|journal=wiley online library|volume=29|pages=775–785|via=}}</ref> |
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Sommaruga et al.(2014) <ref name=":1">{{Cite journal|last=Sommaruga|first=Silvia|date=2014|title=mmobilization of carboxypeptidase from Sulfolobus solfataricus on magnetic nanoparticles improves enzyme stability and functionality in organic media. BMC Biotechnol.|url=http://www.biomedcentral.com/1472-6750/14/82|journal=BMC biotechnologie|volume=14:82|pages=|via=}}</ref>also improved the stability and reaction yield of a well-characterized [[carboxypeptidase]] from S.solfataricus MT4 by magnetic nanoparticles immobilizing the enzyme. |
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=== [[Esterase|Esterases]]/[[Lipase|Lipases]] === |
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A new thermostable extracellular lipolytic enzyme [[Serine protease|serine]] [[arylesterase]] which is originally discovered for their large action in the hydrolysis of [[Organophosphate|organophosphates]] from the thermoacidophilic archaeon ''[[Sulfolobus solfataricus]] P1''<ref>{{Cite journal|last=Park|first=Young-Jun|date=2016|title=PurificationandcharacterizationofanewinduciblethermostableextracellularlipolyticenzymefromthethermoacidophilicarchaeonSulfolobussolfataricusP1|url=http://dx.doi.org/10.1016/j.molcatb.2015.11.023|journal=JournalofMolecularCatalysisB:Enzymatic|volume=124|pages=11-19|via=}}</ref>. |
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=== [[Chaperonin ATPase|Chaperonins]] === |
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In reaction to temperature shock (50.4°C) in [[Escherichia coli|E.Coli]] cells , a tiny warm stun protein (S.so-HSP20) from S.solfataricus P2 has been effectively used to imrove tolerance. <ref>{{Cite journal|last=Li|first=Dong-Chol|date=August 2011|title=Thermotolerance and molecular chaperone function of the small heat shock protein HSP20 from hyperthermophilic archaeon, Sulfolobus solfataricus P2. Cell Stress Chaperones|url=https://doi.org/10.1007/s12192-011-0289-z|journal=Springer|volume=17|pages=103-108|via=}}</ref> |
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In view of the fact that chaperonin Ssocpn (920 kDa), which includes [[Adenosine triphosphate|ATP]], K+ and Mg2 + but has not produced any addtional proteins in S.solfataricus to supply collapsed and dynamic proteins from denatured materials ,it was stored on an ultrafiltration cell, while the renatured substrates were moving through the film.<ref>{{Cite journal|last=Cerchia|first=Laura|date=7 August 1999|title=An archaeal chaperonin-based reactor for renaturation of denatured proteins. Extremophile|url=https://doi.org/10.1007/s007920050001|journal=Springer-Verlag 2000|volume=4|pages=1-7|via=}}</ref> |
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=== [[Liposome|Liposomes]] === |
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Because of its tetraether lipid material, the membrane of extreme thermophilic Archaea is unique in its composition. Archaea lipids are a promising source of liposomes with exceptional stability of temperature and pH and tightness against leakage of solute. Such archaeosomes are possible instruments for the delivery of medicines, vaccines, and genes.<ref>{{Cite journal|last=B. Patel|first=Girishchandra|date=1999|title=Archaeobacterial Ether Lipid Liposomes (Archaeosomes) as Novel Vaccine and Drug Delivery Systems|url=https://doi.org/10.1080/0738-859991229170|journal=Critical Reviews in Biotechnology|volume=19|pages=317-357|via=}}</ref> |
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== References == |
== References == |
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{{Reflist|32em}} |
{{Reflist|32em}} |
Revision as of 21:38, 23 December 2019
Sulfolobus solfataricus | |
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Scientific classification | |
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Species: | S. solfataricus
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Binomial name | |
Saccharolobus solfataricus (Stetter and Zillig 1980) Sakai and Kurosawa 2018
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Saccharolobus solfataricus is a species of thermophilic archaeon. It was transferred from the genus Sulfolobus to the new genus Saccharolobus with the description of Saccharolobus caldissimus in 2018.[1]
It was first isolated and discovered in the Solfatara volcano (which it was subsequently named after) in 1980 by two Germans microbiologists Karl Setter and Wolfram Zillig, in Solfatara volcano (Pisciarelli-Campania, Italy).[2]
However, these organisms are not isolated to volcanoes but are found all over the world in places such as hot springs. The species grows best in temperatures around 80° Celsius, a pH level between 2 and 4, and enough sulfur for solfataricus to metabolize in order to gain energy. These conditions qualify it as an extremophile and it is specifically known as a thermoacidophile because of its preference to high temperatures and low pH levels and it’s also in aerobic and heterotropic categories for its metabolic system.[3] It usually has a spherical cell shape and it makes frequent lobes. Being an autotroph it receives energy from growing on sulfur or even a variety of organic compounds.[4]
Currently, it is the most widely studied organism that is within the Crenarchaeota branch. Solfataricus are researched for their methods of DNA replication, cell cycle, chromosomal integration, transcription, RNA processing, and translation. All the data points to the organism having a large percent of archaeal-specific genes, which showcases the differences between the three types of microbes: archaea, bacteria, and eukarya.
Genome
Sulfolobus solfataricus is the most studied microrganism from a molecular, genetic and biochemical point of view for its ability to thrive in extreme environments; it is easily cultivable in laboratory; moreover, it can exchange genetic material through processes of transformation, transduction and conjugation.
The major motivation for sequencing these microorganisms is because of the thermostability of proteins that normally denature at high temperature. The complete sequence the genome of S. solfataricus was completed in 2001.[5] On a single chromosome, there are 2,992,245 base pairs which encode for 2,977 proteins and copious RNAs. One-third of S. solfataricus encoded proteins have no homologs in other genomes. For the remaining encoded proteins, 40% are specific to Archaea, 12% are shared with Bacteria, and 2.3% are shared with Eukarya.[6] ;33% of these proteins is encoded exclusively in Sulfolobus. A high number of ORFs (open reading frame) are highly similar in Thermoplasma.[7]
Small nucleolar RNAs (snoRNAs) ,already present in eukaryotes, have also been identified in S.Solfataricus and S.acidolcaldarius. They are already known for the role they play in posttranscriptional modifications and removal of introns from ribosomal RNA in Eucarya.[8]
The genome of Sulfolobus is characterised by the presence of short tandem repeats,insertion and repetitive elements, it has a wide range of diversity as it has 200 different ISs insertion sequence elements.
Thermophilic reverse gyrase
The stabilisation of the double helix against denaturation, in the Archaea, is due to the presence of a particular specific thermophilic enzyme,reverse gyrase. It was discovered in hyperthermophilic and thermophilic Archaea and Bacteria .There are two genes in Sulfolobus that each encode a reverse gyrase.[9] It is defined atypical Dna topoisomerases and the basic activity consists in the production of positive supercoils in a closed circular Dna.Positive supercoiling is important to prevent the formation of open complexes. Reverse gyrases are composed of two domains : the first one is the helicase like and second one is the topoisomerase I. A possible role of reverse gyrase could be the use of positive supercoiling to assemble chromatin-like structures. [10] In 1997 scientists discovered another important feature of Sulfolobus : this microrganism contains a type-II topoisomerase, called TopoVI, whose A subunit is homologous to the meiotic recombination factor, Spo11 which plays a predominant role initiation of meiotic recombination in all Eucarya [11][12]
S. solfataricus is composed of three topoisomerases of type I, TopA and two reverse gyrases, TopR1 and TopR2, and one topoisomerase of type II, TopoVI.[13]
Dna binding proteins
In the Phylum Crenarchaeota there are three proteins that bind the minor groove of Dna like histones:Alba, Cren7, and Sso7d, that are modified after the translation process. These are small and have been found in several strains of Sulfolobus but not in other genome.Chromatin protein in Sulfolobus represent 1-5% of the total. They can have both structural and regulatory functions. These look like human HMG-box proteins, because of their influence on genomes, for the expression and the stability, and on epigenetic processes.[14] In species lacking histones they can be acetylated and methylated like eukaryotic histones.[15] [16][17][18] Sulfolobus strains present different peculiar DNA binding proteins, such as the Sso7d protein family. They stabilize the double helix, preventing denaturation at high temperature thus promoting annealing above the melting point. [19]
The major component of archael chromatin is represented by Sac10b family protein known as Alba (Acetylation lowers binding affinity).[20][21]These proteins are small, basic and dimeric nucleic acid-binding proteins.Furthermore, it is conserved in most sequenced archeal genomes. [22] [23]The acetylation state of Alba, as an example, affects promoter access and transcription in vitro , whereas the methylation state of another Sulfolobus chromatin protein, Sso7D, is altered by culture temperature.[24][25]
The work of Wolfram Zillig’s group, representing early evidence of the eukaryotic characteristics of the transcription in Archea, has since made Sulfolobus an ideal model system for transcription studies .Recent studies in Sulfolobus, in addition to other archaeal species, mainly focus on the composition, function and regulation of the transcription machinery in these organisms and on fundamental conserved aspects of this process in both Eucarya and Archaea [26]
DNA transfer
Exposure of Saccharolobus solfataricus to the DNA damaging agents UV-irradiation, bleomycin or mitomycin C induces cellular aggregation.[27] Other physical stressors, such as changes in pH or temperature shift, do not induce aggregation, suggesting that induction of aggregation is caused specifically by DNA damage. Ajon et al.[28] showed that UV-induced cellular aggregation mediates chromosomal marker exchange with high frequency. Recombination rates exceeded those of uninduced cultures by up to three orders of magnitude. Frols et al.[27][29] and Ajon et al.[28] hypothesized that the UV-inducible DNA transfer process and subsequent homologous recombinational repair represents an important mechanism to maintain chromosome integrity. This response may be a primitive form of sexual interaction, similar to the more well-studied bacterial transformation that is also associated with DNA transfer between cells leading to homologous recombinational repair of DNA damage.[citation needed]
Metabolism
Sulfolobus solfataricus is known to grow chemoorganotrophically, in presence of oxygen, on a variety of organic componds such as sugars, alcohols, amino acids and aromatic compounds like phenol.[30]
It uses a modified Entner-Doudroff pathway for glucose oxidation and the resulting pyruvate molecules can be totally mineralized in TCA cycle.[30]
Molecular oxygen is the only known electron acceptor at the end of the electron tranport chain.[31] Other than organic molecules, this Archea species can also utilize hydrogen sulfide[6] and elementar sulfur as electron donors and fix CO2 , possibly by means of HP/HB cycle,[30] making it also capable of living chemoautotrophycally. Recent studies have found also the capability of growing, albeit slowly, oxidizing molecular hydrogen.[1]
Ferredoxin
Ferredoxin is suspected to act as the major metabolic electron carrier in S. solfataricus. This contrasts with most species within the Bacteria and Eukarya, which generally rely on NADH as the main electron carrier. S. solfataricus has strong eukaryotic features coupled with many uniquely archaeal-specific abilities. The results of the findings came from the varied methods of their DNA mechanisms, cell cycles, and transitional apparatus. Overall, the study was a prime example of the differences found in crenarchaea and euryarchaea.[6][32]
Ecology
Habitat
S. solfataricus is an extreme termophile Archea, as the rest of the species of the genus Sulfolobus , it has optimal growth conditions in strong vulcanic activity areas , with hight temperature and very acid pH,[33] these specific conditions are typical of vulcanic area as geyser or theraml springs, infact the most studied countries where microorganism were found are: U.S.A (Yellowstone National Park),[34] New Zeland,[35] Island and Italy, notoriously famous for volcanic phenomena like these. A study conducted by a team of Indonesian scientists has shown the presence of a Sulfolobus community also in the West Java, confirming that high fears, low ph and sulfur presence are necessary conditions for the growth of these microbes.[36]
Soil acidification
S. solfataricus is able to oxidizing sulfur in according to metabolic strategy, one of the products of these reactions is H+ and, consequentially, it’s results in a slowly acidification of surrounding area. Soil acidification increase in place where there are emmissions of pollutants from industrial activity, and this process reduce the number of heterotrophic bacterial involved to decomposition, which are foundamental to recycling organic matter and ultimately to fertilizing soil.[37]
Biotechnologie
Untapping the resource Sulfolobus
Today, in many fields of application, we are interested in using Sulfolobus sulfataricus as a source of thermal stability enzymes for research and diagnostics, as well as in the food, textile and cleanning industries, and the pulp and paper industry.Furthermore, this enzyme is overloaded due to its catalytic diversity, high pH and temperature stability, increased to organic solvents and resistance to proteolysis.[38][39]
At present, tetraester lipids, membrane vesicles with antimicrobial properties, trehalose components, and new β-galactooligosaccharides are coming increasingly important.[40]
The thermostable enzyme β-galactosidase isolated from the extreme thermophile archaebacterial Sulfolobus solfataricus , strain MT-4.
This enzyme utilized on many industrial process of lactose containing fluids by purifying and characterizing for their physicochemical properties.[41]
The industry are interested in stable proteases as well as in many different sulfolobus proteases that have been studied. [42]
An active aminopeptidase associated with the chaperonin of Solfobulus solfataricus MT4 was described.[43]
Sommaruga et al.(2014) [44]also improved the stability and reaction yield of a well-characterized carboxypeptidase from S.solfataricus MT4 by magnetic nanoparticles immobilizing the enzyme.
A new thermostable extracellular lipolytic enzyme serine arylesterase which is originally discovered for their large action in the hydrolysis of organophosphates from the thermoacidophilic archaeon Sulfolobus solfataricus P1[45].
In reaction to temperature shock (50.4°C) in E.Coli cells , a tiny warm stun protein (S.so-HSP20) from S.solfataricus P2 has been effectively used to imrove tolerance. [46]
In view of the fact that chaperonin Ssocpn (920 kDa), which includes ATP, K+ and Mg2 + but has not produced any addtional proteins in S.solfataricus to supply collapsed and dynamic proteins from denatured materials ,it was stored on an ultrafiltration cell, while the renatured substrates were moving through the film.[47]
Because of its tetraether lipid material, the membrane of extreme thermophilic Archaea is unique in its composition. Archaea lipids are a promising source of liposomes with exceptional stability of temperature and pH and tightness against leakage of solute. Such archaeosomes are possible instruments for the delivery of medicines, vaccines, and genes.[48]
References
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{{cite journal}}
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{{cite journal}}
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{{cite journal}}
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- ^ Zillig W, Stetter KO, Janeković D (June 1979). "DNA-dependent RNA polymerase from the archaebacterium Sulfolobus acidocaldarius". European Journal of Biochemistry. 96 (3): 597–604. doi:10.1111/j.1432-1033.1979.tb13074.x. PMID 380989.
- ^ a b Fröls S, Ajon M, Wagner M, Teichmann D, Zolghadr B, Folea M, et al. (November 2008). "UV-inducible cellular aggregation of the hyperthermophilic archaeon Sulfolobus solfataricus is mediated by pili formation" (PDF). Molecular Microbiology. 70 (4): 938–52. doi:10.1111/j.1365-2958.2008.06459.x. PMID 18990182.
- ^ a b Ajon M, Fröls S, van Wolferen M, Stoecker K, Teichmann D, Driessen AJ, et al. (November 2011). "UV-inducible DNA exchange in hyperthermophilic archaea mediated by type IV pili" (PDF). Molecular Microbiology. 82 (4): 807–17. doi:10.1111/j.1365-2958.2011.07861.x. PMID 21999488.
- ^ Fröls S, White MF, Schleper C (February 2009). "Reactions to UV damage in the model archaeon Sulfolobus solfataricus". Biochemical Society Transactions. 37 (Pt 1): 36–41. doi:10.1042/BST0370036. PMID 19143598.
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Further reading
- Fiorentino G, Del Giudice I, Petraccone L, Bartolucci S, Del Vecchio P (June 2014). "Conformational stability and ligand binding properties of BldR, a member of the MarR family, from Sulfolobus solfataricus". Biochimica et Biophysica Acta. 1844 (6): 1167–72. doi:10.1016/j.bbapap.2014.03.011. PMID 24704039.
- de Rosa M, Bemporad F, Pellegrino S, Chiti F, Bolognesi M, Ricagno S (September 2014). "Edge strand engineering prevents native-like aggregation in Sulfolobus solfataricus acylphosphatase". The FEBS Journal. 281 (18): 4072–84. doi:10.1111/febs.12861. PMID 24893801.
- Gamsjaeger R, Kariawasam R, Touma C, Kwan AH, White MF, Cubeddu L (October 2014). "Backbone and side-chain ¹H, ¹³C and ¹⁵N resonance assignments of the OB domain of the single stranded DNA binding protein from Sulfolobus solfataricus and chemical shift mapping of the DNA-binding interface". Biomolecular NMR Assignments. 8 (2): 243–6. doi:10.1007/s12104-013-9492-4. PMID 23749431.
- Wang J, Zhu J, Min C, Wu S (May 2014). "CBD binding domain fused γ-lactamase from Sulfolobus solfataricus is an efficient catalyst for (-) γ-lactam production". BMC Biotechnology. 14: 40. doi:10.1186/1472-6750-14-40. PMC 4041915. PMID 24884655.
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