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Phytophthora mississippiae sp. nov., a New Species Recovered from Irrigation Reservoirs at a Plant Nursery in Mississippi | OMICS International
ISSN: 2157-7471
Journal of Plant Pathology & Microbiology

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Phytophthora mississippiae sp. nov., a New Species Recovered from Irrigation Reservoirs at a Plant Nursery in Mississippi

Xiao Yang1*, Warren E Copes2 and Chuanxue Hong1

1Department of Plant Pathology, Physiology and Weed Science, Hampton Roads Agricultural Research and Extension Center, Virginia Polytechnic Institute and State University, Virginia Beach, Virginia, USA

2Agricultural Research Service, US Department of Agriculture, Thad Cochran Southern Horticultural Laboratory, Poplarville, Mississippi, USA

*Corresponding Author:
Xiao Yang
Department of Plant Pathology, Physiology and Weed Science
Hampton Roads Agricultural Research and Extension Center
Virginia Polytechnic Institute and State University Virginia Beach, Virginia, USA
E-mail: [email protected]

Received date: May 27, 2013; Accepted date: June 28, 2013; Published date: June 30, 2013

Citation: Yang X, Copes WE, Hong C (2013) Phytophthora mississippiae sp. nov., a New Species Recovered from Irrigation Reservoirs at a Plant Nursery in Mississippi. J Plant Pathol Microb 4: 180. doi:10.4172/2157-7471.1000180

Copyright: © 2013 Yang X, et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

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Abstract

A previously unknown Phytophthora species was recovered from irrigation water in Mississippi. This novel species produced both nonpapillate and semipapillate sporangia, and catenulate hyphal swellings. All examined isolates were compatibility type A1. Ornamented oogonia with amphigynous antheridia and plerotic oospores were produced when this novel species was paired with A2 mating type testers of P. cryptogea and P. nicotianae in polycarbonate membrane tests. Sequence analyses of the rDNA internal transcribed spacer (ITS) region and the mitochondrially encoded cytochrome c oxidase 1 (cox 1) gene placed this species in clade 6 of the genus Phytophthora. Based on the morphological, physiological and molecular features, this new species is named as Phytophthora mississippiae sp. nov. The implications of these results are discussed.

Keywords

Phytophthora mississippiae; Irrigation reservoir; Ornamented oogonia

Introduction

The genus of Phytophthora was first described by Heinrich Anton de Bary in 1876 [1]. œPhytophthora was from the Greek word “φυτόνφθορά” which means the plant-destroyer. The name evidences that Phytophthora genus includes a group of destructive plant pathogens. This genus was divided into 10 clades following phylogenetic analyses [2-4]. Among these clades, clade 6 has a strong association with forest and riparian environments [5]. It currently consists of 18 formal species. All were described after the year 2000, except for P. gonapodyides [6], P. humicola [7] and P. megasperma [8]. Clade 6 also includes a number of provisional species such as P. taxon forest soil, P. taxon oaksoil, and P. taxon Pgchlamydo [9], as well as many other undescribed taxa (Hong et al. unpublished).

Several factors have contributed to the recent increase in the number of species in clade 6. First, advancements in molecular biology and sequence analysis provide viable alternatives to morphospecies concepts used in traditional taxonomic systems such as the taxonomy key of Phytophthora species developed by Waterhouse [10]. Accompanying these advancements is identification of definitive characters and phylogenetic analysis tools that have greatly facilitated re-examination of Phytophthora collections and description of new species. For example, P. rosacearum and P. sansomeana were recently separated from the P. megasperma species complex after sequence analyses [11]. P. sp. O-group isolated in the 1990s was formally named as P. inundata [12]. P. taxon Salixsoil first isolated in the 1970s was assigned as P. lacustris [13]. Many newly isolated species in clade 6 such as P. bilorbang [14] and P. gemini [15] were also described by taking advantage of phylogenetic analysis. Second, recent occurrence of sudden oak death (SOD) caused by P. ramorum in the United States [16,17] and forest declines caused by several Phytophthora species in other countries [18,19] has motivated global surveys of natural habitats and waterways for these pathogens. These surveys done in natural environments recovered a number of new species such as P. borealis and P. riparia [20], plus other taxa that belong to clade 6. Third, parallel surveys of irrigation systems have been greatly intensified to address growing concerns over the increasing Phytophthora disease risk as agricultural industries increasingly use recycled water in the light of global water scarcity [21,22]. The surveys in irrigation systems also recovered a number of novel Phytophthora species [23-25] and many new taxa in clade 6 (Hong et al. unpublished).

The objective of this study was to characterize and describe a group of isolates belonging to a previously unknown Phytophthora species recovered from irrigation reservoirs in Mississippi. We describe the morphological, physiological and molecular characters of this new taxon and formally name it as Phytophthora mississippiae sp. nov.

Materials and Methods

Isolation and isolate maintenance

The origin of four Phytophthora mississippiae isolates examined in this study is shown in Table 1. They were recovered from the surface, middle, or bottom of water columns in irrigation reservoirs at an ornamental plant nursery of Mississippi in 2012 by baiting with rhododendron leaves [26,27]. These baits were deployed in the surveyed reservoirs for 7 days then transferred to a laboratory. They were then cut into approximately 3×3 cm2 sections and plated onto PARP selective media (contains pimarcin, ampicillin, rifampicin, and pentachloronitrobenzene). Phytophthora colonies emerging from the edge of baits were hyphal-tipped onto 20% clarified V8 juice agar (CV8A) to obtain pure cultures [1]. Cultures were maintained on CV8A and blocks of fresh agar cultures were transferred into microtubes with sterile distilled water for long-term storage at 15°C. The holotype isolate MYA-4946 was deposited at the American Type Culture Collection in Manassas, Virginia, USA.

Species ITS clade Isolate Location Substrate Date GenBank accession no.
ITS cox 1
Phytophthora mississippiae 6 57J1 Mississippi, USA Irrigation water 2012 KF112850 KF112858
    57J2 Mississippi, USA Irrigation water 2012 KF112851 KF112859
    57J3 T Mississippi, USA Irrigation water 2012 KF112852 KF112860
    57J4 Mississippi, USA Irrigation water 2012 KF112853 KF112861
P. amnicola 6 DH228 Australia Still water 2009 JQ029956 JQ029948
P. asparagi 6 SP326 Michigan, USA Asparagus officinalis 2008 EF185089 n/a *
    CBS121536 The Netherlands Asparagus officinalis n/a n/a JX524163
P. bilorbang 6 CBS161653 Australia Rhizosphere soil of dying Rubus sp. 2012 JQ256377 JQ256375
P. borealis 6 AKWA58.1-0708 Alaska, USA Creek water 2012 HM004232 JQ626625
P. fluvialis 6 MURU 468 Australia River water 2009 JF701436 JF701442
P. gemini 6 CBS123381 The Netherlands Zostera marina 1998 FJ217680 JX262931
P. gibbosa 6 CBS127951 Australia Root soil of dying Acacia pycnantha 2009 HQ012933 HQ012846
P. gonapodyides 6 34A8, CBS55467 United Kingdom Fruit bait 1967 KF112854 KC733448
P. gregata 6 CBS127952 Australia Root soil of dying Patersonia sp. 2009 HQ012942 HQ012858
P. humicola 6 32F8, P3826 Taiwan Soil slurries 1977 KF112855 KF112862
P. inundata 6 30J3, P894 Spain Olea roots 1966 KF112856 KF112863
P. lacustris 6 P245 United Kingdom Salix matsudana 1972 AF266793 JF896561
P. litoralis 6 CBS127953 Australia Root soil of dying Banksia sp. 2008 HQ012948 HQ012866
P. megasperma 6 CBS40272 Washington, D.C. , USA Althaea rosea 1931 HQ643275 n/a
    IMI133317 Australia n/a 1968 n/a AY564194
P. pinifolia 6 CMW26668 Chile Pinus radiata 2007 EU725806 JN935961
P. riparia 6 3-100B9F Oregon, USA Creek water 2006 HM004225 n/a
P. rosacearum 6 22J9, OSU 62 California, USA Cherry n/a KF112857 KF112864
P. thermophila 6 CBS127954 Australia Root soil of dying Eucalyptus sp. 2004 EU301155 HQ012872
P. infestans 1 27A8, KDT-2C Mexico Solanum tuberosum 1992 KC733443 KC733447
P. meadii 2 CBS21988 India Hevea brasiliensis 1987 HQ643268 AY564192
P. sojae 7 28F9, P6497 Mississippi, USA Glycine max 1974 KC733444 AY564162
P. lateralis 8 IMI040503, CBS16842 Oregon, USA Chamaecyparis lawsoniana 1942 AF266804 AY564191
P. aquimorbida 9 40A6 Virginia, USA irrigation reservoir 2006 FJ666127 GQ294536
P. macrochlamydospora 9 33E1, P10264 Australia Glycine max 2003 KC733445 KC733454
Pythium aphanidermatum Pythium P1779 n/a n/a n/a GU983641 n/a
    P2 n/a n/a n/a n/a AY564163

Table 1: Origin and GenBank accession numbers of Phytophthora mississippiae isolates and reference species.

Colony morphology and cardinal temperatures

Ten-day-old colony morphology of the four isolates of P. mississippiae on carrot agar (CA), CV8A, malt extract agar (MEA), and potato dextrose agar (PDA) grown at 20°C in the dark was noted and photographed.

Cardinal temperatures of the four isolates were assessed on CV8A and CA. Agar blocks (5 mm in diameter) taken from actively growing areas of 7-day-old cultures were placed on fresh media at the center of 10-cm Petri dishes. Triplicate Petri dishes per isolate per temperature were placed in the dark at 5, 10, 15, 20, 25, 30, 35, and 40°C. Two perpendicular measurements of each colony were taken after 8 days. This test was repeated. Following the analysis of variance using R statistical software v. 2.15.0 [28], data from repeating tests were pooled together. Radial growths along with their standard errors were plotted against temperature using the gplots package v. 2.11.0 [29] in R.

Morphology of sporangia and gametangia

Sporangia were produced by transferring agar plugs (10×10 mm2) from actively growing area of 10-day-old cultures on CV8A to Petri dishes containing non-sterile, 1.5% soil water extract solution (SWE, 15g of sandy loam soil/1 L distilled water) or filtered, non-sterile pond water. Mature sporangia developed after incubating at room temperature (c. 23°C) under cool-white fluorescent light.

Mating type of these isolates was determined by placing each with an A1 or A2 mating type tester of P. cinnamomi in dual cultures on hemp seed agar (HSA). Selfed sexual structures were produced at room temperature using the polycarbonate membrane method to physically separate P. mississippiae isolates from their reverse mating type testers [30,31]. Several heterothallic species including P. cinnamomi, P. cambivora, P. meadii, P. nicotianae, and P. cryptogea were used as mating type testers.

Sporangia and gametangia were photographed with a Nikon Fujix Digital Camera HC-300Zi connected to a Nikon Labophot-2 microscope. Fifty randomly selected mature sporangia were measured for length and width while 30 gametangia were measured for the size of oogonia, oospores, and antheridia with Image-Pro® Plus v. 5.1.2.53.

DNA extraction, amplification and sequencing

Isolates were grown in 20% V8 juice broth at room temperature for one week. Mycelial masses were harvested and lysed using a FastPrep®-24 system (MP Biomedicals, Santa Ana, CA). DNA was extracted as instructed using the DNeasy® Plant Mini kit (Qiagen, Valencia, CA). Amplifications were performed with forward primer ITS6 and reverse primer ITS4 [2] for the internal transcribed spacer (ITS) region covering ITS1, 5.8S rRNA gene, and ITS2, following previously described reaction mix recipe and PCR program [32]. Primer pair COX4FR was used to amplify the mitochondrial cytochrome c oxidase 1 (cox 1) gene [3]. Sequencing was performed in both directions at the University of Kentucky Advanced Genetic Technologies Center (Lexington, KY) using the same primers. Sequences of both directions were visualized with Finch TV v. 1.4.0. and aligned using Clustal W.

Sequence analyses

Sequences generated in this study were compared with those of all other species in the same clade and species representing other clades (Table 1). Sequences were aligned using Clustal W. Phylogeny reconstruction was conducted in MEGA 5.1 [33] using the Maximum Likelihood method based on the Tamura-Nei model [34] with 1,000 replications of bootstrap.

Results

Colony morphology

The four isolates of P. mississippiae had a similar growth pattern at 20°C on each medium (Figure 1). Colonies had none to sparse aerial mycelia and grew at the greatest rates on CA. The colony pattern on CA was radiate with a smooth edge. Isolates 57J1, 57J3 and 57J4 had a moderate growth rate on CV8A while isolate 57J2 had a slow growth rate. All isolates produced hispid aerial mycelia. Colony pattern on CV8A was radiate to slightly petaloid with a relatively smooth edge. On MEA, all isolates had limited but discernible growth with irregular colony patterns. Isolates had a moderate growth rate on PDA and produced tomentose aerial mycelia. Colony pattern on PDA was petaloid (isolates 57J1, 57J2 and 57J3) to slight cottony (isolate 57J4).

plant-pathology-microbiology-Colony-morphology-isolates

Figure 1: Colony morphology of Phytophthora mississippiae isolates on various media incubated at 20°C for 10 days in the dark: CA=carrot agar; CV8A=20% clarified V8 juice agar; MEA=malt extract agar; PDA=potato dextrose agar.

Cardinal temperatures for vegetative growth

Radial growth rates were different among isolates (P<0.01) but not between repeating experiments (P=0.17). Isolates 57J1, 57J3, and 57J4 had similar growth rates (Figure 2A). Isolate 57J2 grew more slowly than the other isolates at 10 to 30°C on both CV8A and CA (Figure 2B). The optimum temperature for the growth of P. mississippiae was 25°C on CA and 30°C on CV8A. Limited but notable growth was observed at 5 and 35°C. No growth occurred at 40°C. After the experiments were completed, cultures from all temperatures were relocated to room temperature. Additional growth occurred on plates previously maintained at 5°C but not those maintained at 40°C.

plant-pathology-microbiology-Differential-radial-growth

Figure 2: Differential radial growth of Phytophthora mississippiae isolates on carrot agar (CA) and 20% clarified V8 juice agar (CV8A): A. Daily radial growth rates of isolates 57J1, 57J3, and 57J4; B. 57J2.

Sequence analyses and phylogenetic position

GenBank accession numbers of sequences generated in this study and used in the sequence analyses are shown in Table 1. All isolates of P. mississippiae have 818 bp ITS sequences. Isolates 57J1 and 57J2 have an identical ITS sequence, while 57J3 and 57J4 have an identical ITS sequence (Table 2). These two subgroups differ by 3 bp. These ITS sequences of P. mississippiae were distinct from those of all known Phytophthora species. Two species with most similar ITS sequences are P. borealis and P. gonapodyides . P. mississippiae differs from P. borealis (GenBank accession no. HM004232) and P. gonapodyides (GenBank accession no. KF112854) in the ITS sequence by 7 and 8 bp, respectively (Table 2).

Isolate ITS1 ITS2
15 43 44 98 106 173 469 517 553 582 588 608 652 740 744 787
  Phytophthora mississippiae                    
57J1, 57J2 A T A C A C C T C G G C T T G -
57J3, 57J4 A T A C G T T T C G G C T T G -
  Phytophthora borealis                      
AKWA58.1-0708 - T A Y G C T T C S G Y G G G -
  Phytophthora gonapodyides                    
34A8 A A T C G T T G T G A C G T A T

Table 2: Polymorphic nucleotides in the sequences of internal transcribed spacer region (ITS) among Phytophthora mississippiae isolates and the type isolates of P. borealis and P. gonapodyides. Compared to the sequence of P. mississippiae type isolate 57J3, the differential nucleotides of isolates 57J1 and 57J2, P. borealis, and P. gonapodyides are shaded.

The four P. mississippiae isolates have an identical 867 bp cox 1 sequence, which also is distinct from those of all known species. The cox 1 sequence of P. mississippiae differs from two proximal sequences, those of P. thermophila (GenBank accession no. HQ012872) and P. borealis (GenBank accession no. JQ626625) by 30 and 31 bp, respectively.

Sequence analyses of both ITS and cox 1 sequences placed P. mississippiae in clade 6 of the genus Phytophthora [5,9]. The four P. mississippiae isolates form a distinct taxon in the phylogenetic trees based on ITS (Figure 3) and cox 1 (Figure 4) sequences.

plant-pathology-microbiology-maximum-likelihood-phylogenetic

Figure 3: A maximum likelihood phylogenetic tree generated in MEGA 5.1, based on the alignment of ITS sequences with Clustal X. The numbers on branches are bootstrap values (1,000 replicates; values less than 50% are not shown).

plant-pathology-microbiology-maximum-phylogenetic-generated

Figure 4: A maximum likelihood phylogenetic tree generated in MEGA 5.1 based on the alignment of partial cox 1 sequence with Clustal X. The numbers on branches are bootstrap values (1,000 replicates; values less than 50% are not shown).

Taxonomy

Phytophthora mississippiae X. Yang, W. E. Copes, and C. X. Hong., sp. nov.”MycoBank MB804659; Figures 1, 5A-Q, 6A-D.

plant-pathology-microbiology-Morphology-asexual-structures

Figure 5: Morphology of asexual structures of Phytophthora mississippiae: A-G) Nonpapillate, noncaducous sporangia in various shapes; A) An obpyriform to ovoid sporangium; B, C:0Obpyriform sporangia; D) An ovoid sporangium; E) An slightly excentric, ellipsoid sporangium; F) A secondary, ovoid sporangium; G) A secondary, obpyriform sporangium; H) A semipapillate, ovoid sporangium; I) A semipapillate, ellipsoid sporangium; J) A semipapillate sporangium right before releasing zoospores; K) A sporangium releasing zoospores; L) Internal extended proliferation; M) Nesting proliferation; N) Smooth, flat mycelia; O) Coiled mycelia; P) Swollen mycelia; Q) Catenulate hyphal swellings.
Bars=10 μm.

plant-pathology-microbiology-Morphology-gametangia-Phytophthora

Figure 6: Morphology of gametangia of Phytophthora mississippiae: A, B) Selfing gametangia induced by P. cryptogea; A) An oogonium with an ornamented surface and a tapered base, a bi-celled, amphigynous antheridium, and two immature gametangia; B) An oogonium with ornamented surface and tapered base; C, D) Selfing gametangia induced by P. nicotianae; C) A plerotic oospore with a cylindroid, amphigynous antheridium; D) Three different sized oogonia.
Bars=10 μm.

Phytophthora mississippiae produced abundant sporangia in 1.5% SWE after 15 hours under light. Sporangia were mostly ovoid to obpyriform (Figures 5A-D, F-H, J). It occasionally produced slight ellipsoid sporangia (Figures 5E, I). Sporangia were noncaducous, mostly nonpapillate (Figures 5A-G) and sometimes semipapillate (Figures 5H-J). Primary sporangia were terminal and averaged 60.5 µm in length and 31.7 µm in width. Secondary lateral sporangia were observed on the mycelial plug after submersion in SWE for more than 40 hours. Nested and extended internal proliferation was common (Figures 5L, M). Sporangial characteristics among four P. mississippiae isolates are summarized in Table 3. Mycelia were flat (Figure 5N), coiled (Figure 5O), or swollen (Figure 5P). Hyphal swellings were commonly elongated with irregular shapes, especially in aged cultures (>30-dayold). Catenulate, globose hyphal swellings were frequently observed in both fresh and aged cultures (Figure 5Q). Chlamydospores were not observed.

Character Isolate Species average
57J1 57J2 57J3 57J4
Shape (%)          
ovoid to obpyriform 86 93 96 90 92
slightly ellipsoid 12 7 4 2 6
distorted 1 - - 8 2
Papilla (%)          
nonpapillate 66 70 53 69 64
semipapillate 33 30 47 31 36
Size range (µm) 47.3-70.0 x 21.1-43.3 48.8-64.3 x 26.8-38.6 55.4-71.9 x 28.6-41.9 47.3-77.3 x 20.4-37.1 47.3-77.3 x 20.4-43.3
Average size (µm) 61.5 ± 7.2 x 34.0 ± 3.5 57.4 ± 3.9 x 31.1 ± 2.5 62.6 ± 3.8 x 34.9 ± 3.2 60.3 ± 7.2 x 26.8 ± 3.4 60.4 ± 6.0 x 31.3 ± 4.5
L:W ratio 1.82 1.85 1.80 2.27 1.96

Table 3: Morphological variations of sporangial characters among isolates of Phytophthora mississippiae in this study.

Phytophthora mississippiae is self-sterile. Gametangia were produced in dual cultures where P. mississippiae isolates were paired with an A2 mating type tester of P. cinnamomi suggesting that all four isolates examined in this study are A1. In the polycarbonate membrane test, gametangia were produced by isolates 57J3 and 57J4 after 50-day-breeding when paired with A2 mating type testers of P. cryptogea (Figures 6A, B) and P. nicotianae (Figure 6C, D). Oogonia had characteristic ornamented protuberances on the surface and oogonial wall was pigmented to golden-brown with maturation (Figures 6A-D). Many oogonia had a tapered base (Figures 6A, B, D). Oogonial diameter averaged 38.2 µm. Plerotic oospores averaged 34 µm in diameter (Figures 6A-D). All antheridia were amphigynous (Figures 6A-D) and averaged 19.5 µm depth and 14.3 µm width. Sometimes bicellular antheridia were produced (Figure 6A).

Holotype

ATCC MYA-4946 (exo-type: 57J3) from irrigation water of a nursery reservoir, Mississippi, USA, February, 2012.

Etymology

mississippiae refers to the state of Mississippi where this new species was isolated.

Habitat

Irrigation water of an ornamental plant nursery, Mississippi, USA.

Discussion

This study characterized a novel species of Phytophthora morphologically, physiologically and phylogenetically then named it as P. mississippiae. This is the first and critical step to understanding the biology, ecology and economic significance of any novel species. The description of P. mississippiae will help the first responders in diagnosing the disease caused by this new species. It also will reduce misidentification of high-impact pathogens like P. ramorum [17] and P. kernoviae [35].

Phytophthora mississippiae can be readily distinguished from all known Phytophthora species by its morphological and molecular characters. Within the genus Phytophthora, only 5 species, P. alni [36], P. cambivora [6], P. gibbosa [5], P. katsurae [37], and this new species, P. mississippiae produce ornamented oogonia with bullate protuberances. P. mississippiae is easily separated from three homothallic species, P. alni, P. gibbosa and P. katsurae [5,31,36,37] by its heterothallism. Both P. cambivora and P. mississippiae are heterothallic, but they can be separated by the papillation of sporangia and presence of hyphal swellings. P. mississippiae produces both nonpapillate and semipapillate sporangia, while P. cambivora produces only nonpapillate sporangia [31]. P. mississippiae also frequently produces catenulate hyphal swellings, while P. cambivora typically does not. Similarly, P. mississippiae can be easily differentiated from other clade 6 species including P. borealis, P. thermophila, and P. gonapodyides in cox 1 sequences (>30 bp difference).

Like many other species in clade 6, the economic importance of P. mississippiae is not known at this point. Many clade 6 species are abundant in natural habitats and frequently recovered from natural water and soil environments, but usually do not cause apparent disease symptoms on plants [38]. Only a few clade 6 species have been found to cause diseases on agricultural and horticultural plants [5]. Examples include P. asparagi which causes root rot of asparagus [39] and P. megasperma which causes crown rot of hollyhock [8]. A saprophytic lifestyle for many species in this clade may play an important role in decomposing plant debris [38]. Unlike many other clade 6 species initially detected in natural environments, P. mississippiae was first recovered from irrigation water in a plant production facility. It is possible that P. mississippiae was carried into agricultural irrigation water systems from surrounding habitats through flash flood runoff that occurred in this area during heavy rains. This hypothesis is supported by the fact that this new species was found only in Mississippi but not in any of nursery irrigation systems surveyed in Virginia during the past 14 years and in Alabama during the past 2 years. Nevertheless, investigations into its origin, pathogenicity and host range are warranted.

Acknowledgements

This research was supported in part by grants from USDA/NIFA (2005-51101- 02337, 2010-51181-21140). We thank Mrs. Patricia Richardson for her assistance in maintaining the cultures and submitting PCR products for DNA sequencing during the study. Our thank extends to Mr. Xitong Li for his help with processing and editing figures for this manuscript.

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