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Incidence and multiplex PCR based detection of trichothecene chemotypes of Fusarium culmorum isolates collected from freshly harvested Maize kernels in Southern India

Abstract

Hundred Fusarium culmorum strains, isolated from freshly harvested maize grain samples from Southern parts of India, were incubated in czapek-dox medium and analyzed for trichothecene (DON/NIV) production. The mPCR assay was standardized targeting trichothecene metabolic pathway genes viz., Tri6, Tri7, Tri13 for detection of trichothecene (DON/NIV) chemotypes and rDNA gene for specific detection of F. culmorum species. Primers for targeted genes were designed and used to predict whether these isolates could produce deoxynivalenol/nivalenol, 94 isolates were able to produce DON/NIV by mPCR assay. Chemical analysis of DON/NIV was carried out for mPCR positive isolates by high performance-thin layer chromatography (HPTLC). To check the practical usefulness of developed mPCR assay, 150 field samples of maize were evaluated and results were compared with conventional HPTLC method. Out of 150 samples, 34% samples stayed as a positive for NIV contamination whereas 44% were found to have deoxynivalenol contamination. Moreover, mPCR results are equivocally matched with the HPTLC chemical analysis for field samples. Chemotyping of F. culmorum isolates were reported for the first time from India, and highlights the important potential of F. culmorum to contaminate maize with DON/NIV.

deoxynivalenol; nivalenol; multiplex PCR assay; HPTLC


FOOD

RESEARCH PAPER

Incidence and multiplex PCR based detection of trichothecene chemotypes of Fusarium culmorum isolates collected from freshly harvested Maize kernels in Southern India

M. Venkataramana; P. Shilpa; K. Balakrishna; H.S. Murali; H.V. Batra

Defence Food Research Laboratory, Microbiology Devision, Sidartha Nagar, Mysore, Karnataka, India

Send correspondence to Send correspondence to: M. Venkataramana Defence Food Research Laboratory, Microbiology Devision Sidartha Nagar, Mysore, 570011Karnataka E-mail: ramana.micro@gmail.com

ABSTRACT

Hundred Fusarium culmorum strains, isolated from freshly harvested maize grain samples from Southern parts of India, were incubated in czapek-dox medium and analyzed for trichothecene (DON/NIV) production. The mPCR assay was standardized targeting trichothecene metabolic pathway genes viz., Tri6, Tri7, Tri13 for detection of trichothecene (DON/NIV) chemotypes and rDNA gene for specific detection of F. culmorum species. Primers for targeted genes were designed and used to predict whether these isolates could produce deoxynivalenol/nivalenol, 94 isolates were able to produce DON/NIV by mPCR assay. Chemical analysis of DON/NIV was carried out for mPCR positive isolates by high performance-thin layer chromatography (HPTLC). To check the practical usefulness of developed mPCR assay, 150 field samples of maize were evaluated and results were compared with conventional HPTLC method. Out of 150 samples, 34% samples stayed as a positive for NIV contamination whereas 44% were found to have deoxynivalenol contamination. Moreover, mPCR results are equivocally matched with the HPTLC chemical analysis for field samples. Chemotyping of F. culmorum isolates were reported for the first time from India, and highlights the important potential of F. culmorum to contaminate maize with DON/NIV.

Key words: deoxynivalenol, nivalenol, multiplex PCR assay, HPTLC.

Introduction

The genus Fusarium is a common fungal contaminant of many economically important field crops and food products, which causes a major contamination in human and animal nutrition. Fusarium sp. infects many important food grains, such as maize, wheat, barley, rice, millet, oat and rye, and produce highly toxic secondary metabolites known as mycotoxins. The major classes of Fusarium mycotoxins are trichothecenes and fumonisins. According to the type of trichothecene production, some Fusarium species, like F. culmorum and other species have been divided into two chemotypes: (i) the nivalenol chemotype, which includes isolates producing nivalenol and fusarenone X, and (ii) the deoxynivalenol chemotype, which includes isolates producing deoxynivalenol and acetyldeoxynivalenol (Langseth et al., 1999; Muthomi et al., 2000). Trichothecenes can cause wide range of acute and chronic effects in humans and animals through ingestion of food and feed prepared from cereal crops contaminated with the toxins (Mello et al., 1999). The effects include skin inflammation, digestive disorders, trachycardia, oedema and haemorrhages in several internal organs, haemolytic disorders, impairment of immune disorders and nervous disorders (IARC, 1993).

Contamination of maize grains with trichothecenes is a common problem throughout the World, especially in temperate regions like India (Janardhana et al., 1999; Venkataramana et al., 2011). In Southern India, maize is grown under different ecological conditions and is harvested with fairly high trichothecene contaminations (Janardhana et al., 1999). Recent reports indicate that maize is prone to fungal infection during the pre and post harvest period (Bilgrami et al., 1980; Sinha, 1990). Vasanthkumar (Vasanthkumar, 1986) studied the infection of maize by field and storage moulds during pre and post harvest practices in relation to seed-borne fungal diseases of maize. Thimmappaiah et al. (1987) reported the natural occurrence of Fusarium toxins such as T-2 toxin, deacetoxyscirpenol and zearalenone in peanut, sorghum and maize from Mysore districts of Southern India. Pre-harvest succession of fungi in ripening maize grains has been reported by Banerjee et al. (Beyer et al., 2005).

The usual methods for chemotyping of Fusarium isolates are high performance liquid chromatography (HPLC) or gas chromatography/ mass spectroscopy (GS/MS) analysis of extracts from substrates such as maize artificially inoculated with Fusarium (Sugiura et al., 1990; Muthomi et al., 2000). These methods are commonly applied due to their high sensitivity and specificity. However, these methods are rather labour-intensive and require sophisticated instrumentation and skilled operators. Recent studies are focusing genotypic identification of toxigenic fungi through molecular methods. DNA based methods that rely on the amplification of the genes involved in the biosynthesis of trichothecenes also are available. Specific PCR primers have been developed to the specific genes (Tri5, Tri6, Tri7 and Tri13) which are involved in trichothecene metabolism (Venkataramana et al., 2011; Lee et al., 2001). Some of the genes have been sequenced and found to be functional in NIV-producing isolates and nonfunctional in DON-producing isolates (Lee et al., 2002, 2001; Chandler et al., 2003).

The distribution of each chemotype/genotype varies by geographic region. Thus, strains of F. culmorum with DON and NIV chemotype/ genotype are known from several countries, including UK (Jennings et al., 2004), Germany (Muthomi et al., 2000), the Netherlands and Norway (Langseth et al., 1999), Italy (Gang et al., 1998), France (Bakan et al., 2001), USA (Mirocha et al., 1994), Canada (Abramson et al., 2001). However in India, we are first time reporting incidence of trichothecene chemotypes of F. culmorum on maize kernels by multiplex PCR method.

In the present study a novel mPCR method was developed for detection of trichothecene chemotypes of F. culmorum. Developed method was successfully evaluated in terms of sensitivity, specificity and reliability on to artificially contaminated samples as well as contaminated field samples of maize.

Materials and Methods

Sampling area

A total of 150 freshly harvested maize kernel samples were randomly collected from Karnataka and Andhra Pradesh, two districts from each state viz., Kusalnagara and Mysore districts of Karnataka; Srikakulam and Vizianagaram districts of Andhra Pradesh, India. Collected samples were stored at 4 ºC for further analysis of mycoflora and toxin detection.

Isolation and identification of moulds from infected maize grains

Isolation of mycoflora

F. culmorum and other fungal genera were isolated from the infected maize grains using Potato Dextrose Agar (PDA) media. The morphological identification of Fusarium species were followed by the previous reports of Nelson et al. (1983). The pure cultures of Fusarium was maintained on SNA plates and stored at 4 ºC for analysis of toxins.

DNA extraction

DNA was extracted from pure cultures of Fusarium sp., using commercially available DNA extraction kits (QUIAZEN, Gambh).

Isolation of DNA from contaminated food grains

Twenty grams of contaminated food sample was ground in coffee grinder for 90 s and then 0.2 g ground grain was mixed in 1 mL lysis buffer (100 mM Tris-HCl, 50 mM EDTA, 150 mM NaCl and 1% SDS) and homogenized by gentle mixing and kept it for water bath at 60 ºC for 10 min. Samples were centrifuged at 12000 x g for 5 min and 500 µL of supernatant was mixed with 150 µLof 5 M potassium acetate and incubated on ice for 10 min. After centrifugation a 400 µL of supernatant was mixed with 300 µL of ice cold isopropanol to precipitate the DNA, the resulting pellet was washed with 70% ethanol, dried under air and dissolved in 50 µLof Tris-EDTA (pH 8.0).

Development of primers and PCR analysis

Designing of primers

DNA sequences were analysed and aligned by Clustal method. Primers were designed using the aligned gene bank database sequences viz., Tri6, Tri7, Tri13 and rDNA genes for the specific detection of nivalenol and deoxynivalenol producing F. culmorum. Total of four primer pairs were designed using Gene runner software (http://www.generunner.com). Primer sequences are listed in Table 1. Before standardizing mPCR protocol, all designed primers were evaluated on to array of fungal species to check the specificity and sensitivity.

Multiplex PCR assay

Multiplex PCR was carried out for DON and NIV producing F. culmorum in an Eppendorf master cycler gradient (Hamburg, Germany) with a reaction volume of 30 µL. The amplification mixture consisted of template DNA (1.0 µL), MgCl2 (2.0 mM), 1X PCR buffer (Sigma), dNTP mix (200 µM, MBI, Fermentas), Taq polymerase (1 unit, Sigma) and primer pairs specific to the targeted genes Tri6, Tri7,Tri13 and rDNA were added at a concentration of 100 nM, 150 nM, 200 nM and 50 nM, respectively. The PCR cycling conditions were carried out with an initial denaturation at 94 ºC for 4 min, followed by 30 cycles of 94 ºC for 1 min, 58 ºC for 1 min and 72 ºC for 1.5 min, with a final extension of 72 ºC for 8min.

Specificity and sensitivity of mPCR on artificially contaminated maize grains

The specificity of the mPCR primers was determined against different organisms shown in (Table 2). Sterile maize grains (5 g) were experimentally spiked with F. culmorum spore suspensions at different concentrations (1x105, 1x104, 1x103 and 1x102 cfu g-1). Negative controls were kept without inoculation of spores. All the samples were enriched for two days, further DNA was isolated and analysed by mPCR assay.

Application of mPCR on field samples

Analysis of field samples

Maize samples were collected from various fields of Andhra Pradesh and Karnataka, India and processed as described earlier and all of these samples were subjected to mPCR assay and toxins are analyzed by HPTLC.

Chemical analysis of DON and NIV

Extraction and cleanup

Briefly, 50 g of the well ground sample was extracted with 250 mL of acetonitrile-water (60:40, v/v) using high speed blending for 2 min. The extract was filtered through Whatman No. 4 filter paper and an equal volume of ethyl acetate was added to the filtrate and separated the lower chloroform fraction and evaporated to dryness. Dried compound was diluted with PBS and passed through immunoaffinity columns (VICAM, USA) for clean-up. After washing with water, DON /NIV were eluted with methanol. These extracts further used for HPTLC analysis.

HPTLC detection

High performance thin layer chromatography (HPTLC) technique was used to detect the specific chemotypes of (DON /NIV) F. culmorum. Chromatography was carried out on 10 x 10 cm precoated silica gel HPTLC plates (Merck). Test samples and standards were applied with automatic TLC sampler (ATS III) from CAMAG (Muttenz, Switzerland), with a 50 mm run length using: chloroform + methanol + water (9+1+0.2, v/v/v.) as mobile phase. Fluorescence detection was carried out by postchromatographic derivatization with 10% aluminium chloride (Sigma) in methanol-water mixture. The plate was immersed in the derivatization solution using a dipping device III (CAMAG) and heated for 20 min at 110 ºC. The plate was then scanned at 366/ > 400 nm with a densitometer TLC Scanner 3 (CAMAG) using a slit dimension of 5.0 x 0.5 mm and scanning speed of 40 mm s-1 (18). DON and NIV standards (Sigma) at a concentration of 0.1 mg/mL in methanol: water (1:1) was used as positive controls for HPTLC detection.

Results

Incidence of mycotoxigenic Fusarium culmorum and other fungi

A total of 150 Fusarium isolates were identified from the maize samples of the present study. Out of 150 fungal isolates, 100 isolates were identified with F. culmorum morphologically (45 isolates from Karnataka and 55 isolates from Andhra Pradesh) and remaining 50 isolates from other species including F. sporotrichioides, F. verticillioides and F. proliferatum (Table 3).

Multiplex PCR assay application and chemical analysis of pure cultures of fungi

Primer concentrations (100 nM of Tri6, 150 nM of Tri7, 200 nM of Tri13 and 50 nM of rDNA) and annealing temperature (58 ºC) were standardized to get a uniform amplification of all the genes targeted for mPCR assay (Figure 1). Out of 150 Fusarium isolates, 100 were showed positive signal for rDNA gene specific to F. culmorum (94 toxigenic to DON/NIV and remaining were non toxigenic by mPCR). However, 54 and 34 strains of them were positive for DON and NIV respectively, and rest of the 7 strains were stayed as negative for the chemical analysis by HPTLC.


Contamination studies

The detection limit for deoxynivalinol and nivalenol producing F. culmorum strains from spiked samples by mPCR was 1x103 cfu g-1 maize grains. Samples tested with initial fungal load of 1x103 cfu g-1 and above concentrations following 48 h enrichment at 30 ºC were positive for both toxins.

mPCR and chemical analysis of field samples

Out of 150 maize samples collected for mPCR studies, 78% samples were showed positive for toxigenic Fusarium species. However, only 34% of the total analysed samples were positive for NIV and 44% positive for DON chemotypes. Toxin analysis by HPTLC providing equivocal results with mPCR for both the groups of toxins.

Discussion

It would be more meaningful if analytical systems are made available for low cost, simple to use qualitative and for quantitative assessments of the mycotoxigenic fungi and mycotoxins present in the different food matrices. Conventional methods for the detection of Fusarium based on sporodochia with abundant macroconidia on the chaff surface is time consuming and laborious, however, PCR assays have proven to be very useful and sensitive where sporodochia are absent or in poorly developed state (Nicholson et al., 1998). Multiplex PCR assays have been applied for the detection of air samples and for diseased plant, animal and human tissues for the presence of bacteria, parasites, viruses and fungi (Yenny et al., 2009; Mohd et al., 2010). In this study, we attempted a mPCR assay with an objective to obtain simultaneous detection of trichothecene chemotypes of F. culmorum spp. that are commonly associated with Fusarium disease.

A total of 150 Fusarium isolates originated from Andhra Pradesh and Karnataka, India were assayed by mPCR/HPTLC for their mycotoxin chemotypes. Results were showed that 100 strains have the rDNA gene specific to F. culmorum. Additionally mPCR amplification of Tri6, Tri7 and Tri13 alleles suggests that 94% of the F. culmorum isolates are able to produce DON/NIV. Some other researchers observed that, the same NIV and DON accumulation by F. culmorum in wheat grains (Kammoun et al., 2009; Lobna et al., 2010). However, to our knowledge in India, we are reporting first time DON/NIV chemotypes in maize kernels. In the present study, DON chemotypes were more aggressive when compared to NIV chemotypes of F. culmorum. The higher incidence of DON chemotypes may be due to intra specific variation of gene clusters of F. culmorum strains (Bakan et al., 2001). The findings of Jennings et al. (2004) were confirmed our results, that DON chemotypes dominance in F. culmorum strains. Whereas, Lauren et al. (1992) and Lee et al. (2002) reported contradictory results that NIV dominants in F. culmorum.

The four DNA amplicons scored (Figure 1) were serve as a diagnostic tool for the early detection of trichothecene chemotypes of F. culmorum. The 300 bp amplicon is signifies the rDNA gene specific to F. culmorum, 546 bp region of Tri6 gene is specific to all trichothecene producing Fusarium species (both type A and type B) whereas, 900 bp Tri7 gene region specific to NIV chemotype and 1000 Bp region of Tri13 gene is specific to DON chemotypes of F. culmorum was used in this study.

Results of the molecular assays (mPCR) were confirmed by chemical analysis by HPTLC. Thus HPTLC conducted on 94 mPCR positive F. culmorum isolates revealed that 54 isolates were positive for DON and 33 were positive for NIV toxin, whereas, 7 strains were negative for chemical analysis. The variation in mPCR and HPTLC analysis is not unexpected since Quarta et al. (2005) and Ramana et al., (2011) compared the molecular analysis with chemical analysis for toxigenic Fusarium species and made the similar kind of findings. Thus while a positive trichothecene genotype indicates the potential for trichothecene biosynthesis, only a test for the toxin itself can be used to determine if and how much toxin a strain has produced. In vitro, DON/NIV may be produced by utilizing very different culture conditions such as whole grain, solid substrate fermentation, or liquid cultures using a defined minimal medium. Our results corroborate that growth conditions greatly influence the amount of mycotoxin produced. trichothecene biosynthesis may be regulated by temperature (Ramirez et al., 2006), relative humidity (Beyer et al., 2005), and substrate composition (ONeill et al., 1993). Results lead to the conclusion that in vitro assays could not appropriate to predict production of DON in the field as suggested by Gang et al. (1998). The physiology of plant-hosts and pathogenesis of the strain itself may further influence mycotoxin accumulation under field conditions. However, in the case of field samples mPCR results are equivocally matched with the chemical analysis. So, the newly developed mPCR assay is an alternative for the time consuming and laborious conventional culture methods for early assessment of trichothecene chemotypes of F. culmorum from field samples. The present research has demonstrated that, the occurrence of F. culmorum in Southern India (Andhra Pradesh and Karnataka) is dominant; it may due to cool climatic conditions and high moisture and rainfalls. Global variation in DON/NIV production by isolates of F. culmorum and distribution of these isolates geographically and by host are important in Plant pathology and food safety and security.

Conclusion

High levels of toxigenic F. culmorum incidence in maize samples demonstrates the need for better surveillance and monitoring by policy makers or food toxicologists to reduce the exposure of human and animal life to toxic compounds produced by fungi.

Acknowledgments

Authors are thankful to the director DFRL, Mysore, for his providing necessary facilities to carry out the work.

Submitted: October 29, 2011

Approved: July 23, 2012

All the content of the journal, except where otherwise noted, is licensed under a Creative Commons License CC BY-NC.

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  • Send correspondence to:

    M. Venkataramana
    Defence Food Research Laboratory, Microbiology Devision
    Sidartha Nagar, Mysore, 570011Karnataka
    E-mail:
  • Publication Dates

    • Publication in this collection
      09 Oct 2013
    • Date of issue
      2013

    History

    • Received
      29 Oct 2011
    • Accepted
      23 July 2012
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