Morphological and molecular differentiation of the pectinase producing fungi Penicillium expansum and Penicillium griseoroseum

Cardoso, Patrícia Gomes; Queiroz, Marisa Vieira de; Pereira, Olinto Liparini; Araújo, Elza Fernandes de

doi:10.1590/s1517-83822007000100015

Cited by 24 publications

(17 citation statements)

References 30 publications

(21 reference statements)

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“…c Inhibition zone between P. frequentans and C. beticola Kawano et al (1999) who noted that P. frequentans produced high levels of extracellular pectinases after 24 h of incubation in submerged culture. Moreover, many researches have shown the ability of different Penicillium species to produce some enzymes, such as P. italicum (Alana et al 1990), pectolytic molds (Fawole and Odunfa 1992), P. viridicatum RFC3 (Silva et al 2002), P. roqueforti (Pericin et al 2007), and P. expansum (Cardoso et al 2007). From these results, it is clear that there was a correlation between enzyme activity and the antagonistic ability for each isolate.…”

Section: Pectinase and Cellulase Activitymentioning

confidence: 91%

Evaluation of certain Penicillium frequentans isolates against Cercospora leaf spot disease of sugar beet

El-Fawy

El-Sharkawy

Abo-Elyousr

2018

Egypt J Biol Pest Control

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The impact of six local isolates of Penicillium frequentans recovered from healthy sugar beet (Beta vulgaris L.) leaves was evaluated against Cercospora beticola, the causal pathogen of Cercospora sugar beet leaf spot under laboratory and field conditions. In in vitro studies, all the six isolates were able to inhibit the mycelial growth of C. beticola with variation in their antagonistic capability. P. frequentans isolates produce pectinase and cellulase at different degrees. There was a correlation between enzyme activity and the antagonistic ability for each isolate. The high antagonistic ability isolates had the most enzyme activity. In field studies, some adhesives such as agar, starch flour, white glue, gum, and commercial adhesive (Triton Mok) were added to conidia spore suspensions of P. frequentans at 1% to improve conidial adhesion to sugar beet plant surface. Data also showed that all adhesives increased (P = 0.05) the efficiency of the spore suspension of P. frequentans to control the disease. The starch flour at 1% gave a significant reduction in disease severity from 43.23 to 10.42% pre-infection and from 43.23 to 10.52% post-infection. The application of P. frequentans led to improved root yield and the sugar percent of sugar beet crop in two tested seasons.

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Section: Pectinase and Cellulase Activitymentioning

confidence: 91%

Evaluation of certain Penicillium frequentans isolates against Cercospora leaf spot disease of sugar beet

El-Fawy

El-Sharkawy

Abo-Elyousr

2018

Egypt J Biol Pest Control

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“…DQ325456-DQ325457 T. mycotoxinivorans (Molnar et al, 2004) and strain R-4272 (Hickey et al, 2009); G. loubieri (Scorzetti et al, 2002 (Wu et al, 2003) 99.7% DQ325458-DQ325459 P. italicum (AJ250548), P. commune (Buzina et al, 2003), P. expansum (Cardoso et al, 2007), P. solitum var. crustosum (Vega et al, 2006;Bakys et al, 2009) (EF634415), and P. griseoroseum (Cardoso et al, 2007) (Wu et al, 2003) and A. awamori (Nikkuni et al, 1996) 99.9% DQ325463 A. niger (Buzina et al, 2003;Haugland et al, 2004;Huitron et al, 2008), A. awamori and A. foetidus (Haugland et al, 2004) 99.1% a profiles did not consider restriction fragments under 70 bp.…”

Section: Characterization Of Fungal Culturable Diversity: Microbial Amentioning

confidence: 99%

“…crustosum (Vega et al, 2006;Bakys et al, 2009) (EF634415), and P. griseoroseum (Cardoso et al, 2007) (Wu et al, 2003) and A. awamori (Nikkuni et al, 1996) 99.9% DQ325463 A. niger (Buzina et al, 2003;Haugland et al, 2004;Huitron et al, 2008), A. awamori and A. foetidus (Haugland et al, 2004) 99.1% a profiles did not consider restriction fragments under 70 bp. several toxic metabolites, which present potent immunosuppressive, genotoxic, cytotoxic, and apoptotic effects (Latge, 2001;Boudra and Morgavi, 2005).…”

Section: Characterization Of Fungal Culturable Diversity: Microbial Amentioning

confidence: 99%

Characterization of cultivated fungi isolated from grape marc wastes through the use of amplified rDNA restriction analysis and sequencing

et al. 2010

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Microbial assessment of grape marc wastes, the residual solid by-product of the wine-industry, was performed by identifying phylogenetically the fungal culturable diversity in order to evaluate environmental and disposal safety issues and to discuss ecological considerations of applications on agricultural land. Fungal spores in grape marc were estimated to 4.7 x 10(6) per g dry weight. Fifty six fungal isolates were classified into eight operational taxonomic units (OTUs) following amplified ribosomal DNA restriction analysis (ARDRA) and colony morphology. Based on 18S rRNA gene and 5.8S rRNA gene-ITS sequencing, the isolates representing OTUs #1, #2, #3, and #4, which comprised 44.6%, 26.8%, 12.5%, and 5.3%, respectively, of the number of the total isolates, were identified as Aspergillus fumigatus, Bionectria ochroleuca, Haematonectria haematococca, and Trichosporon mycotoxinivorans. The isolates of OTU#5 demonstrated high phylogenetic affinity with Penicillium spp., while members of OTUs #6 and #7 were closer linked with Geotrichum candidum var. citri-aurantii and Mycocladus corymbifer, respectively (95.4 and 97.9% similarities in respect to their 5.8S rRNA gene-ITS sequences). The OTU#8 with a single isolate was related with Aspergillus strains. It appears that most of the fungal isolates are associated with the initial raw material. Despite the fact that some of the species identified may potentially act as pathogens, measures such as the avoidance of maintaining large and unprocessed quantities of grape marc wastes in premises without adequate aeration, together with its suitable biological treatment (e.g., composting) prior to any agriculture-related application, could eliminate any pertinent health risks.

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“…Morphological variations and molecular differentiation methods like rRNA gene sequences, RAPD, AFLP or RFLP are being used to discriminate the strains of same genera or species and mutants [21,[23][24][25][26]. The objective of this study was to generate the mutant strain of S. johnsonii having significant improvement in CoQ 10 content and to differentiate it from wild type strain, based on cultural and microscopic morphology, rRNA gene sequences and physiological attributes.…”

Section: Introductionmentioning

confidence: 99%

Morphological and Molecular Differentiation of Sporidiobolus johnsonii ATCC 20490 and Its Coenzyme Q10 Overproducing Mutant Strain UF16

et al. 2014

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Coenzyme Q 10 (CoQ 10 ) is an industrially important molecule having nutraceutical and cosmeceutical applications. CoQ 10 is mainly produced by microbial fermentation and the process demands the use of strains with high productivity and yields of CoQ 10 . During strain improvement program consisting of sequential induced mutagenesis, rational selection and screening process, a mutant strain UF16 was generated from Sporidiobolus johnsonii ATCC 20490 with 2.3-fold improvements in CoQ 10 content. EMS and UV rays were used as mutagenic agents for generating UF16 and it was rationally selected based on atorvastatin resistance as well as survival at free radicals exposure. We investigated the genotypic and phenotypic changes in UF16 in order to differentiate it from wild type strain. Morphologically it was distinct due to reduced pigmentation of colony, reduced cell size and significant reduction in mycelial growth forms with abundance of yeast forms. At molecular level, UF16 was differentiated based on PCR fingerprinting method of RAPD as well as large and small-subunit rRNA gene sequences.Rapid molecular technique of RAPD analysis using six primers showed 34 % polymorphic fragments with mean genetic distance of 0.235. The partial sequences of rRNAgene revealed few mutation sites on nucleotide base pairs. However, the mutations detected on rRNA gene of UF16 were less than 1 % of total base pairs and its sequence showed 99 % homology with the wild type strain. These mutations in UF16 could not be linked to phenotypic or genotypic changes on CoQ 10 biosynthetic pathway that resulted in improved yield. Hence, investigating the mutations responsible for deregulation of CoQ 10 pathway is essential to understand the cause of overproduction in UF16. Phylogenetic analysis based on RAPD bands and rRNA gene sequences coupled with morphological variations, exhibited the novelty of mutant UF16 having potential for improved CoQ 10 production.

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Morphological and molecular differentiation of the pectinase producing fungi Penicillium expansum and Penicillium griseoroseum

Cited by 24 publications

References 30 publications

Evaluation of certain Penicillium frequentans isolates against Cercospora leaf spot disease of sugar beet

Evaluation of certain Penicillium frequentans isolates against Cercospora leaf spot disease of sugar beet

Characterization of cultivated fungi isolated from grape marc wastes through the use of amplified rDNA restriction analysis and sequencing

Morphological and Molecular Differentiation of Sporidiobolus johnsonii ATCC 20490 and Its Coenzyme Q10 Overproducing Mutant Strain UF16

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