Characterization and in Plant Detection of Bacteria That Cause Bacterial Panicle Blight of Rice ()
1. Introduction
Rice production in the southern United States has a long history of loss to panicle blighting of unknown etiology. The losses caused by bacterial panicle blight (BPB) could be as high as 70%, including reduced yield and poor milling [1] . Significant yield losses from BPB have been experienced in the rice-producing regions of the Southern United States, including Louisiana, Texas and Arkansas in 1996, 1997, 2000, and the most recently, in 2010 [2] . Currently, this disease has affected rice production in many countries of Asia, Africa, South and North America; it is a typical example of the shifting from a minor plant disease to a major disease due to the changes of environmental conditions [3] . The symposiums of BPB often appear during the rice heading stage and are pronounced when rice is grown under high night temperature and frequent rainfalls predisposing rice to diseases outbreak [4] .
Rapid detection and accurate identification of pathogens in plant are critical steps to prevent pathogens dissemination. Pathogen identification based on colony morphology or disease symptoms is difficult, time-consuming and unreliable because of the secondary infection by necrotrphic fungi and the similarity among Burkholderia spp. For example, B. glumae, B. plantarii, and B. gladioli were known to infect rice plants causing similar symptoms [5] . Additionally, proliferation of B. glumae and B. plantarii were found to suppress B. gladioli in rice seeds [6] . Interactions among B. glumae, B. gladioli, B. plantarii and other unknown microorganisms often result in different outcomes of crop damage. For example, B. glumae was found to be responsible for the decrease of grain weight, floret sterility, inhibition of seed germination and reduction of stands in rice seedlings dependent on the outcome of the interactions with other bacteria and the environmental factors such as temperature and drought [7] .
Previous studies have identified abundance of strains of B. glumae including some highly virulent strains that caused 50% to 75% yield reduction [8] [9] . Additionally, it was predicted that the B. glumae strains in different rice-production regions have some undefined differences in their genome and virulence [3] . Furuya et al. (1997) demonstrated that the extent of virulence of B. glumae strains can be accurately estimated by the use of hypersensitive cell death on tobacco [10] . However, virulence characteristics of B. glumae isolated from rice, and distribution of the causal agent of bacterial panicle blight (BPB) in rice plants have not been clearly demonstrated. Tobacco hypersensitivity is a fast and convenient way to screen bacterial cultures for pathogenicity. It works particularly well for Pseudomonas but can be variable for Xanthomonas and Ralstonia. Some Xanthomonads may require some tweaking of the environmental conditions for the tobacco grown in [11] [12] , and the response may take up to four days [13] [14] . Erwinia amylovora and some of the coryneform bacteria will also cause a hypersensitive response. Ralstonia solanacearum cause various results depending on the race. Race 1 results in chlorosis after two days, race 2 induces a typical hypersensitive response in one day and race 3 results in chlorosis after two to eight days [15] .
The genetic identity of Burkholderia species has been analyzed by polymerase chain reaction (PCR) using 16S rRNA sequences [16] [17] . The discriminatory power of 16S rRNA is too restricted to reveal the detailed phylogenetic relationships among B. plantarii, B. glumae and B. gladioli because of extremely slow rate of evolution of the 16S rRNA gene, it cannot discriminate closely related microorganisms [18] . On the other hand, the genes encoding the β-subunit polypeptide of DNA gyrase (gyrB) estimated to evolve much faster than the 16S rRNA gene that can be used to develop a specific and sensitive detection method [18] to distinguish among Burkholderia species [5] . Therefore, specific primers developed from the gyrB sequences should be reliable for specific detection and identification of B. glumae and B. gladioli in rice materials.
The aims of this study were to 1) isolate and identify the bacterial panicle blight (BPB) pathogen with culture media; 2) verify the causal agent of BPB with PCR; 3) evaluate virulence with tobacco plants; and 4) determine distribution of B. glumae in plants with PCR.
2. Material and Methods
2.1. Isolation and Identification of the Pathogen
During a 2015 cropping season, 178 naturally infected immature rice panicles with bacterial Panicle blight (BPB) symptoms were collected from growing counties of Arkansas (Supplemental Table S1 and Figure 1). Seeds and florets with discoloration and blanked panicles were collected in paper bags and kept in a refrigerator at 4˚C until processing. Seeds were disinfected with 10% sodium hypochlorite for 1 min and rinsed three times with sterile distilled water then left to dry on a sterile filter paper. Disinfected seeds were directly plated on a semi-selective media of CCNT (containing 2 g of yeast extract, 1 g of polypepton, 4 g of inositol, 10 mg of cetrimide, 10 mg of chloramphenicol, 1 mg of novobiocin, 100 mg of chlorothalonil and 18 g of agar in 1000 ml of distilled water, and adjusted to pH 4.8) [19] . From each individual sample 30 seeds were planted on two petri dishes using 15 seeds per dish. Those dishes were sealed using a Para film and incubated at 38˚C for 3 to 5 days. The bacterial colonies on these dishes were examined for their morphological characteristics compared with our reference strains of B. glumae. The typical features for bacterial Panicle blight (BPB) on artificial detection media (CCNT) are yellowish white, round, smooth and swollen colonies with a diffusible yellow pigment [19] . Single colonies from each culture plate were collected with a flamed bacteriological loop and
Figure 1. Arkansas rice production county map showing the location of BPB samples collected. Samples collected from 9 rice producing counties of Arkansas as indicated by round cycle dots (please make better figure, it was unclear for me to me to read the name of counties).
streaked on King B medium [20] , incubated at 38˚C for 48 hr, and then stored in Cryo-vial tubes at −80˚C in 30% glycerol. Each isolate was given a culture number.
2.2. Verification of the Causal Agent of Bacterial Panicle Blight (BPB) with PCR
The presence of B. glumae was identified with PCR using a pair of primers to detect specific DNA fragments corresponding to the gyrB nucleotide sequences, glu-FW (5’-GAAGTGTCGCCGATGGAG-3’) and glu-RV (5’-CCTTCACCGA CAGCACGCAT-3’) [5] . Similar primer pairs of gli-FW (5’-CTGCGCCTGG TGGTGAAG-3’) and gli-RV (5’-CCGTCCCGCTGCGGAATA-3’) were also used to amplify DNA fragments corresponding to the gyrB nucleotide sequences of B. gladioli [5] . PCR amplification was initiated for 20 µl containing 1 µl of template DNA with denaturation at 94˚C for 2 min: followed by 35 cycles at 94˚C for 1 min, 63˚C for 1 min and 72˚C for 1 min and 72˚C for 10 min as final extension. Aliquots (10 µl) of each PCR products were loaded onto horizontal electrophoresis on a 2% Tris-acetate-EDTA (TAE) agarose gel (Promega) at 80 V for 90 min. Gels were stained with Syber safe for detection of 530 bp, and 479 bp DNA fragments corresponding to the gryB nucleotide sequences of B. glumae and B. gladioli, respectively [5] . A 1-kb ladder (Invitrogen Co.) was used to predict the fragment size of PCR products. However B. plantarii and other Burkholdria spp. are not included with this study because they are not detected as important disease causing pathogen in USA.
2.3. Distribution of B. glumae in Plants with PCR
To study distribution of B. glumae ten naturally infected rice plants were uprooted from the production fields and brought to a laboratory. Root, stem, sheath, leaf, chuff and seed were collected individually and cleaned with water. These plant parts were disinfected with 1% sodium hypochlorite for 1 min, then rinsed three times with sterile distilled water, and left to dry on a sterile filter paper. Disinfected plant parts were cut to a 1 cm long piece except the seeds that were placed directly on artificial detection (CCNT) media in petri dishes in an incubator at 38˚C for 3 to 5 days. DNA was extracted from these plant parts using a DNeasy Plant Mini Kit (Qiagen, Carlsbad, CA, USA), and from bacteria DNA grow on plate media using a UltraClean Microbial DNA Isolation Kit (MO BIO Laboratories, Qiagen, Carlsbad, CA, USA), respectively.
2.4. Virulence Evaluation with Tobacco Plants
All forty-three isolates identified to be B. glumae were tested for their pathogenicity level with tobacco as described by Furuya et al. [10] . Specifically, tobacco plants (Nicotinaa bethanamiana) were grown to 8 to 9 leaves in approximately 4 weeks after sowing in the greenhouse with a day time temperature ranging between 37˚C to 41˚C and 75% to 90% relative humidity (RH). Inocula were placed on a King’s B agar (KBA) plates incubated at 38˚C for 48 h, then harvested with a sterile cotton swab and suspended in a test tube containing 9 mL of sterile distilled water, and concentration of bacterial suspension were adjusted to be about 108 CFU/mL for inoculation. Three to five tobacco seedlings with the fully expanded leaves were inoculated by injecting at least 3 leaves with 0.5 ml of bacterial suspension using 1 mL sterile syringes and control leaves were injected with sterile distilled water. The control with water did not cause any symptoms one week after injection. The diameters of the lesion of cell death were measured one week after inoculation using four-category disease scale described in Table 1. Large area of necrosis is an indicator for highly virulent strains. After disease
Table 1. Scoring system for tobacco seedling based on the level of hypersensitive reaction to each isolates of B. glumae in greenhouse inoculation tests and number of isolates falling into each category.
aAssigned rating based on necrosis on tobacco leaves one week after injection. bPredicted pathogenicity based on lesion of necrosis on tobacco leaves one week after injection.
scoring, bacteria strains were re-isolated from the diseased tobacco plant to complete Koch’s postulates [21] .
3. Results
3.1. Isolation and Morphological Identification of the Pathogen
Initial symptoms of the bacterial Panicle blight (BPB) caused by B. glumae were observed on the panicles of the rice plant. Infected panicles with a dark brown discoloration and heavily infected panicles with upright due to blanking were basic characteristics to collect panicle samples from 9 rice producing counties of Arkansas. A total of 178 rice panicle samples were collected (Supplemental Table S1). Seeds and Florets from each collected samples were plated on a semi-selective medium and incubated at a temperature range of 38˚C - 40˚C for 5 days. The colony characteristics of these samples were compared with our reference strains of B. glumae. About 41% (73 samples) showed similar morphological characteristics to reference strain which is yellowish white, round, smooth and swollen colonies with a diffusible yellow pigment [19] as shown in Table 2. Isolates which have all other morphological characteristics but lacked pigment production also grow well on artificial detection media (CCNT) but excluded from this study since it has been reported that this types of strains are not pathogenic to rice [22] .
3.2. Verification of the Causal Agent of Bacterial Panicle Blight (BPB) with PCR
The identity of seventy-three isolate of bacterial was also confirmed using B. glumae and B. gladioli-specific PCR amplification [5] . An approximately 530 bp DNA fragments of gryB were amplified for 45 isolates indicating that only 62% out of 73 isolates belongs to B. glumae and the remaining twenty-eight isolates
Table 2. Total numbers, their morphological and molecular identification of samples with respective of the counties.
did not react with B. glumae-specific primers. On the contrary, no fragments were amplified using B. gladioli-specific primer pairs (Table 3).
3.3. Virulence Evaluation with Tobacco Plants
Reaction to tobacco revealed that all 45 isolates tested are pathogenic at different virulence level (Table 3). About 31 isolates (69%) of the 45 isolates tested were highly virulent (Figure 2(a)), while nine isolates (20%) moderately virulent. The remaining isolates categorized as weakly virulent isolates whereas plants injected with sterile distilled water remained healthy with no visible hypersensitivity reaction on the leaves (Figure 2(b)). Koch’s postulates were confirmed by reisolating from inoculated tobacco leaves and then grow them on a semi-selective media (CCNT) for B. glumae (data not shown) Pathogenic B. glumae isolates produced a yellow pigment, identified as toxoflavin, while non-pathogenic strains did not [22] . Accordingly, all forty five isolates tested for their virulence level reislolated from tobacco, and all produced a yellow pigment, which indicated that they are still pathogenic B. glumae bacteria.
3.4. Distribution of B. glumae in a Plant
Ten naturally infected rice plants were removed from a rice paddy and different plants were plated on semi-selective media (CCNT). B. glumae were isolated from seed followed by stem and sheath at low concentration level of yellow pigment. However, roots and leaves did not show any visible yellow pigment on semi-selective media (CCNT) (Figure 3). Pathogen identification was confirmed by PCR using B. glumae-specific primer pair with DNA extracted from individual plant parts (root, stem, leaf, sheath, chaff, and seed). PCR products with predicted sizes were obtained from DNA extracted from seed and chaff. No PCR products were amplified from roots and leaves of rice plant but low level of amplification observed for stem and sheath (Figure 4).
4. Discussion
Bacterial Panicle blight (BPB) is an emerging bacterial disease that causes significant crop loss worldwide. Characterization of the causal agent for BPB and in plant detection pathogen is an important prerequisite to manage BPB. In the present study, 45 disease samples out of the total 178 from commercial rice fields in the state of Arkansas, USA were determined due to B. glumae. None of the disease samples were caused by B. gladioli suggesting that B. glumae is the causal agent for Bacterial Panicle blight (BPB) in Arkansas. The fact that many non-B. glumae were isolated from diseased tissue needs further exploration to see if any uncharacterized microorganism can contribute the development of the syndrome and potential ecological relationships with B. glumae. It is well known that the development of disease symptoms and severity of any plant disease not only depends on virulence of the strain, but also on environmental factors, particularly weather conditions. Symptoms typically caused by B. glumae were
Table 3. Results of virulence level tested by inoculation of Isolates into tobacco leaves to determine pathogenicity level and PCR reaction for two primer sets.
aH indicates no visible reaction, 1, weakly virulent, 2, moderately virulent, 3, highly virulent one week after injection respectively. bglu-FW/glu-RV indicates primers specifically to B. glumae and gli-FW/gli-RV indicates primers specifically to B. gladioli, respectively. Yes indicates PCR product produced and No indicates no PCR amplicon.
Figure 2. Photographic presentation of hypersensitive necrosis on tobacco leaves caused by B. glumae. A. typical necrosis one week after injection with B. glumae, B. One week after tobacco leaves infiltrated with sterile distilled water. W indicated that water was injected.
Figure 3. Photographic presentation of morphology of rice plant parts on Semi specific medium (CCNT). RT indicates roots, ST from stem, CF from Chaff. LF from leaf, SH from sheath, SD from seed, respectively.
panicle blighting with floret discoloration (with a gray-brown color), usually on the lower half of the developing grain, with a clear deep brown border followed
Figure 4. Photographic presentation of PCR amplification of 530-bp product for B. glumae using a pair of primers to detect specific DNA fragments corresponding to the gyrB nucleotide sequences. Samples collected from indicated from different parts of infected rice plants M indicates 1 kilobase ladder, Bg indicates PCR product from B. glumae DNA as positive control, RT indicates DNA from roots, LF from leaf, ST from stem, SH from sheath, CF from Chaff, SD from seed and Co indicates water, respectively.
by sterility or partial filling of the florets causing the panicles to stand erect [23] , [24] . However, all samples examined in the present study were with these symptoms but some of samples found to be other microorganism but not B. glumae and/or B. gladioli. Our study clearly demonstrated that symptom of bacterial Panicle blight (BPB) was not sufficient to identify the causal agent of this disease.
Apparently, it is challenge to differentiate pathogens that are closely related physiologically and taxonomically by the symptoms they produce and by their growth on selective media. A good identification scheme depends not only on developing a satisfactory resolution level of methods, but also on the group of bacteria studied [25] [26] [27] . Semi specific medium (CCNT) is useful for rough screening for bacteria that cause BPB by visualization of unique yellow pigment as indicative of toxoflavin producing bacteria. In the present study we showed that unknown bacteria other than B. glumae and B. gladioli producing similar yellow pigment suggesting that Semi specific medium (CCNT) alone was not sufficient for positive identification of both bacteria. It is fully possible that other unknown bacteria in rice seeds can produce toxoflavin that needs to be further investigated in order to understand their pathogenicity and their bio-control potentials for managing bacterial Panicle blight (BPB) and other rice diseases. In the future, a defined culture medium specifically to B. glumae and B. gladiolia will need to be developed.
We have not found B. gladioli in all diseased samples from Arkansas except B. glumae. To our knowledge, the present study provides the first experimental evidence of B. glumae as the major cause of bacterial Panicle blight (BPB) in Arkansas. This is consistent with that the major causal agent of BPB was B. glumae whereas B. gladioli was less virulent in other geographic regions [28] . In the present study, different isolates of B. glumae show different levels of pathogenicity based on different hypersensitive reaction patterns on tobacco leaves suggesting that there exist genomic and virulence levels variation in Arkansas B. glumae isolates. Forty-five isolates had a hypersensitivity index ranging from weakly to highly sensitive reaction (Table 3). The majority of them caused large necrosis on tobacco suggest that these Arkansas isolates are highly virulent.
5. Conclusion
In summary, we showed that accurate identification of the causal agent for bacterial Panicle blight (BPB) is challenging, and cross-referencing among two or more detection methods is desirable to ensure that the causal agent can be positively identified. We learned that once you suspect the symptom of rice plant tissue damaged by BPB, the next plausible step is to examine seeds derived from diseased rice plants. If possible, the disease tissues should be obtained from vegetative stage before flowering to localize pathogen in stem and/or sheaths. In contrast, because leaves and roots are not a favorable residence for the B. glumae as compared to seed, stem and sheath; therefore, it will not be useful to detect pathogen in leaves and roots. Additionally, we demonstrated that there exhibits difference in virulence among B. glumae and these characterized isolates can be used to screen genetic resistance to bacterial Panicle blight (BPB). Together, our findings are useful for plant quarantine and bacterial Panicle blight (BPB) pathogen identification; ultimately these new knowledge will be useful to manage this emerging agronomically important rice disease worldwide.
Acknowledgements
The authors thank Scott Belmar, Tibebu Gebremariam of Rice Research and Extension Center, UA, AR and Tracy Bianco of USDA Agriculture Research Service Dale Bumpers National Rice Research Center for their excellent technical supports. This project was supported by Arkansas Rice Research Promotion Board.
Supplemental
Note: Isolates that showed yellow pigment on semi-selective media (CCNT) indicated by Yes but if they did not detected using specific primers for B. glumae and B. gladioli using PCR they will be indicated with No. That means morphologically similar but not B. glumae and B. gladioli because PCR is more specific detection than morphology.