Polyhydroxyalkanoate (PHA) Polymer Accumulation and
Autor: | Teresa R. de Kievit, Nidhi Shah, Jocelyn Plouffe, David B. Levin, Riffat I. Munir, Parveen K. Sharma |
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Rok vydání: | 2018 |
Předmět: |
0301 basic medicine
Siderophore Polymers and Plastics 030106 microbiology Mutant relA/spoT Pseudomonas chlororaphis PA23 rpoS Article lcsh:QD241-441 phz- and prn- mutants 03 medical and health sciences chemistry.chemical_compound lcsh:Organic chemistry Gene expression Phenazine Regulatory mutants Regulator gene biology Chemistry Polyhydroxyalkanoates Wild type pha gene expression Biocontrol General Chemistry Pseudomonas chlororaphis biology.organism_classification 6. Clean water gacS 3. Good health Pyrrolnitrin Biochemistry |
Zdroj: | Polymers Volume 10 Issue 11 Polymers, Vol 10, Iss 11, p 1203 (2018) |
ISSN: | 2073-4360 |
Popis: | Pseudomonas chlororaphis PA23 was isolated from the rhizosphere of soybeans and identified as a biocontrol bacterium against Sclerotinia sclerotiorum, a fungal plant pathogen. This bacterium produces a number of secondary metabolites, including phenazine-1-carboxylic acid, 2-hydroxyphenazine, pyrrolnitrin (PRN), hydrogen cyanide, proteases, lipases and siderophores. It also synthesizes and accumulates polyhydroxyalkanoate (PHA) polymers as carbon and energy storage compounds under nutrient-limited conditions. Pseudomonads like P. chlororaphis metabolize glucose via the Entner-Doudoroff and Pentose Phosphate pathways, which provide precursors for phenazine production. Mutants defective in phenazine (PHZ PA23-63), PRN (PA23-8), or both (PA23-63-1) accumulated higher concentrations of PHAs than the wild-type strain (PA23) when cultured in Ramsay&rsquo s Minimal Medium with glucose or octanoic acid as the carbon source. Expression levels of six pha genes, phaC1, phaZ, phaC2, phaD, phaF, and phaI, were compared with wild type PA23 by quantitative real time polymerase chain reaction (qPCR). The qPCR studies indicated that there was no change in levels of transcription of the PHA synthase genes phaC1 and phaC2 in the phz- (PA23-63) and phz- prn- (PA23-63-1) mutants in glucose medium. There was a significant increase in expression of phaC2 in octanoate medium. Transcription of phaD, phaF and phaI increased significantly in the phz- prn- (PA23-63-1) mutant. Mutations in regulatory genes like gacS, rpoS, and relA/spoT, which affect PHZ and PRN production, also resulted in altered gene expression. The expression of phaC1, phaC2, phaF, and phaI genes was down-regulated significantly in gacS and rpoS mutants. Thus, it appears that PHZ, PRN, and PHA production is regulated by common mechanisms. Higher PHA production in the phz- (PA23-63), prn- (PA23-8), and phz- prn- (PA23-63-1) mutants in octanoic medium could be correlated with higher expression of phaC2. Further, the greater PHA production observed in the phz- and prn- mutants was not due to increased transcription of PHA synthase genes in glucose medium, but due to more accessibility of carbon substrates and reducing power, which were otherwise used for the synthesis of PHZ and PRN. |
Databáze: | OpenAIRE |
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