User:S4361440: Difference between revisions
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===Higher order taxa=== | ===Higher order taxa=== | ||
Cellular organisms – Bacteria – Firmicutes – Negativicute – Veillonellales – Veillonellaceae – Veillonella | Cellular organisms – Bacteria – Firmicutes – Negativicute – Veillonellales – Veillonellaceae – Veillonella | ||
===Species=== | ===Species=== | ||
Species name: Veillonella parvula | Species name: ''Veillonella parvula'' <sup>[[#References|[1]]]</sup> | ||
Type strain: DSM 2008 | Type strain: DSM 2008 <sup>[[#References|[1]]]</sup> | ||
==Description and significance== | ==Description and significance== | ||
The French scientists Veillon and Zuber first discovered | The French scientists Veillon and Zuber first discovered ''Veillonella parvula'' in 1898 <sup>[[#References|[2]]]</sup>. V. ''parvula'' is an anaerobic bacterium that has a gram negative cell wall <sup>[[#References|[2]]]</sup>. It is in the form of cocci, usually grown in pairs and it is commonly found in both the supra- and subgingival plaque, as well as the gastrointestinal tract <sup>[[#References|[3]]]</sup>. V. ''parvula'' is one of few bacterial species that is able to be cultured. It does not play a functional role within the human body but has been shown to cause disease on rare occasions. It is important to study V. ''parvula'' as it plays a significant role in the natural microbial food chain, and while V. ''parvula'' rarely causes disease, recent research has found that V. ''parvula'' may assist in the pathogenicity of other bacterial pathogens <sup>[[#References|[4]]]</sup>. | ||
==Genome structure== | ==Genome structure== | ||
The V. | The V. ''parvula'' strains Te3T has a circular chromosome with a length of 2,132,142bp. There were 1,929 predicted genes from which 1,859 coded for proteins. It has a CG content of 38% and contains 15 pseudogenes. 73% of genes were assigned a putative function and the remaining 27% of genes were annotated as hypothetical proteins <sup>[[#References|[3]]]</sup>. | ||
==Cell structure and metabolism== | ==Cell structure and metabolism== | ||
While V. | While V. ''parvula'' are non-motile and cannot adhear it surfaces itself, it is able to attach to specific surface structures present on other cells, often mediated by lectin-carbohydrate interactions <sup>[[#References|[5]]]</sup>. These connections between different bacterial species form a biofilm which provides nutrients and protection for the bacteria. | ||
V. | As V. ''parvula'' has a gram-negative cell wall it has much less peptidoglycan than gram-positive bacteria and it has a cell membrane, as well as an outer membrane. While V. ''parvula'' is a gram-negative bacterium and has lipopolysaccharides, it is more closely related to gram-positive species such as ''Sporomusa'', ''Megasphaera'' or ''Selenomonas'' as they all share the unusual presence of cadaverine and putrescine in their cell wall. A characteristic feature of V. ''parvula'' is the presence of plasmalogens such as plasmenylserine and plasmenylethanolamine as major constituents of the cytoplasmic membrane. These ether lipids replace phospholipids and play an important role in the regulation of membrane fluidity <sup>[[#References|[6]]]</sup>. | ||
V. ''parvula'' have an unusual metabolism where they use methylmalony-CoA decarboxylase to convert the free energy derived from decarboxylation reactions into an electrochemical gradient of sodium ions <sup>[[#References|[7]]]</sup>. They utilize the metabolic end products of co-existing carbohydrate-fermenting bacteria <sup>[[#References|[8]]]</sup>. V. ''parvula'' is unable to use glucose and other carbohydrates for fermentation and is unable to grow on succinate as a sole carbon source however it can decarboxylate succinate during fermentation of malate or lactate. | |||
==Ecology== | ==Ecology== | ||
V. | V. ''parvula'' is an anaerobic bacterium which is located in both the supra- and subgingival plaque, as well as in the gastrointestinal tract. V. ''parvula'' plays a significant role in the natural microbial food chain but does not usually interact directly with the host <sup>[[#References|[3]]]</sup>. | ||
==Pathology== | ==Pathology== | ||
V. | V. ''parvula'' does not usually cause disease as it is an opportunistic pathogen however, in rare cases it has been found to cause endocarditis, meningitis and osteomyelitis <sup>[[#References|[2]]]</sup>. Endocarditis is an infection of the heart which occurs when V. ''parvula'' makes its way into the blood stream and to the heart where it attaches to damaged areas of the heart. Meningitis occurs when V. ''parvula'' passes through the blood brain barrier and is then able to infect areas in the brain and spinal cord. Osteomyelitis occurs when V. ''parvula'' travels through the blood stream and infects bone <sup>[[#References|[2]]]</sup>. | ||
==Application to biotechnology== | ==Application to biotechnology== | ||
V. ''parvula'' has not been involved in any bioengineering or biotechnology research, however it has developed resistance against some antibiotics. V. ''parvula'' shows resistance to erythromycin (>25 μg/ml), kanamycin (>25 μg/ml), tetracycline (>25 μg/ml) and gentamicin (>25 μg/ml) and it is susceptible to cephalotin (1.6 μg/ml), penicillin G (0.4 μg/ml) and clindamycin (0.1 μg/ml) <sup>[[#References|[9]]]</sup>. | |||
==Current research== | ==Current research== | ||
Current research involves the pathogenicity of duel-species biofilms compared to mono-species biofilms. For example, a study investigated the influences of the most dominant Cystic Fibrosis pathogen Pseudomonas aeruginosa and V. parvula during a biofilm associated infection process. It found that the presents of V. parvula supports the growth of P. aeruginosa at the site of infection. In addition, significantly higher levels of P. aeruginosa was recovered from tissue that was coinfected with both bacterial species compared to tissue that was monoinfected with P. aeruginosa. This suggests that while V. | Current research involves the pathogenicity of duel-species biofilms compared to mono-species biofilms. For example, a study investigated the influences of the most dominant Cystic Fibrosis pathogen ''Pseudomonas aeruginosa'' and V. ''parvula'' during a biofilm associated infection process <sup>[[#References|[4]]]</sup>. It found that the presents of V. ''parvula'' supports the growth of P. ''aeruginosa'' at the site of infection. In addition, significantly higher levels of P. ''aeruginosa'' was recovered from tissue that was coinfected with both bacterial species compared to tissue that was monoinfected with P. ''aeruginosa.'' This suggests that while V. ''parvula'' is rarely thet direct cause of disease, it may be facilitating the pathogenicity of other bacterial pathogens <sup>[[#References|[4]]]</sup>. | ||
==References== | ==References== | ||
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8.[http://www.sciencedirect.com.ezproxy.library.uq.edu.au/science/article/pii/0003996970900312 Gibbons, R.J., Nygaard, M. (1970) Interbacterial aggregation of plaque bacteria. Archives of Oral Biology 15:1397,IN1339-1400,IN1339.] | 8.[http://www.sciencedirect.com.ezproxy.library.uq.edu.au/science/article/pii/0003996970900312 Gibbons, R.J., Nygaard, M. (1970) Interbacterial aggregation of plaque bacteria. Archives of Oral Biology 15:1397,IN1339-1400,IN1339.] | ||
9. [http://aac.asm.org.ezproxy.library.uq.edu.au/content/1/2/148 Martin, W.J., Gardner, M., Washington, J.A. II. (1972) In Vitro Antimicrobial Susceptibility of Anaerobic Bacteria Isolated from Clinical Specimens. Antimicrobial Agents and Chemotherapy 1:148.] | |||
<references/> | <references/> | ||
This page is written by Ashley de Klerk for the MICR3004 course, Semester 2, 2016 | This page is written by Ashley de Klerk (43614404) for the MICR3004 course, Semester 2, 2016 |
Latest revision as of 02:19, 23 September 2016
Name Ashley de Klerk Bench C Date 13 Aug 2016 [1]
Classification
Higher order taxa
Cellular organisms – Bacteria – Firmicutes – Negativicute – Veillonellales – Veillonellaceae – Veillonella
Species
Species name: Veillonella parvula [1]
Type strain: DSM 2008 [1]
Description and significance
The French scientists Veillon and Zuber first discovered Veillonella parvula in 1898 [2]. V. parvula is an anaerobic bacterium that has a gram negative cell wall [2]. It is in the form of cocci, usually grown in pairs and it is commonly found in both the supra- and subgingival plaque, as well as the gastrointestinal tract [3]. V. parvula is one of few bacterial species that is able to be cultured. It does not play a functional role within the human body but has been shown to cause disease on rare occasions. It is important to study V. parvula as it plays a significant role in the natural microbial food chain, and while V. parvula rarely causes disease, recent research has found that V. parvula may assist in the pathogenicity of other bacterial pathogens [4].
Genome structure
The V. parvula strains Te3T has a circular chromosome with a length of 2,132,142bp. There were 1,929 predicted genes from which 1,859 coded for proteins. It has a CG content of 38% and contains 15 pseudogenes. 73% of genes were assigned a putative function and the remaining 27% of genes were annotated as hypothetical proteins [3].
Cell structure and metabolism
While V. parvula are non-motile and cannot adhear it surfaces itself, it is able to attach to specific surface structures present on other cells, often mediated by lectin-carbohydrate interactions [5]. These connections between different bacterial species form a biofilm which provides nutrients and protection for the bacteria.
As V. parvula has a gram-negative cell wall it has much less peptidoglycan than gram-positive bacteria and it has a cell membrane, as well as an outer membrane. While V. parvula is a gram-negative bacterium and has lipopolysaccharides, it is more closely related to gram-positive species such as Sporomusa, Megasphaera or Selenomonas as they all share the unusual presence of cadaverine and putrescine in their cell wall. A characteristic feature of V. parvula is the presence of plasmalogens such as plasmenylserine and plasmenylethanolamine as major constituents of the cytoplasmic membrane. These ether lipids replace phospholipids and play an important role in the regulation of membrane fluidity [6].
V. parvula have an unusual metabolism where they use methylmalony-CoA decarboxylase to convert the free energy derived from decarboxylation reactions into an electrochemical gradient of sodium ions [7]. They utilize the metabolic end products of co-existing carbohydrate-fermenting bacteria [8]. V. parvula is unable to use glucose and other carbohydrates for fermentation and is unable to grow on succinate as a sole carbon source however it can decarboxylate succinate during fermentation of malate or lactate.
Ecology
V. parvula is an anaerobic bacterium which is located in both the supra- and subgingival plaque, as well as in the gastrointestinal tract. V. parvula plays a significant role in the natural microbial food chain but does not usually interact directly with the host [3].
Pathology
V. parvula does not usually cause disease as it is an opportunistic pathogen however, in rare cases it has been found to cause endocarditis, meningitis and osteomyelitis [2]. Endocarditis is an infection of the heart which occurs when V. parvula makes its way into the blood stream and to the heart where it attaches to damaged areas of the heart. Meningitis occurs when V. parvula passes through the blood brain barrier and is then able to infect areas in the brain and spinal cord. Osteomyelitis occurs when V. parvula travels through the blood stream and infects bone [2].
Application to biotechnology
V. parvula has not been involved in any bioengineering or biotechnology research, however it has developed resistance against some antibiotics. V. parvula shows resistance to erythromycin (>25 μg/ml), kanamycin (>25 μg/ml), tetracycline (>25 μg/ml) and gentamicin (>25 μg/ml) and it is susceptible to cephalotin (1.6 μg/ml), penicillin G (0.4 μg/ml) and clindamycin (0.1 μg/ml) [9].
Current research
Current research involves the pathogenicity of duel-species biofilms compared to mono-species biofilms. For example, a study investigated the influences of the most dominant Cystic Fibrosis pathogen Pseudomonas aeruginosa and V. parvula during a biofilm associated infection process [4]. It found that the presents of V. parvula supports the growth of P. aeruginosa at the site of infection. In addition, significantly higher levels of P. aeruginosa was recovered from tissue that was coinfected with both bacterial species compared to tissue that was monoinfected with P. aeruginosa. This suggests that while V. parvula is rarely thet direct cause of disease, it may be facilitating the pathogenicity of other bacterial pathogens [4].
References
References examples
1.LPSN
- ↑ MICR3004
This page is written by Ashley de Klerk (43614404) for the MICR3004 course, Semester 2, 2016