Introduction
Sweet potato, Ipomoea batatas (L.) Lam, is a perennial plant of the Convolvulaceae family, native to northwestern South America 6,16. It is ranked among the 10 most important food crops worldwide, with a production of 89,487,835 tons in an area of 7,400,472 hectares in 2020 8. The major sweet potato production areas are located in China and around the Great Lakes of East Africa, but the crop is also important in many other countries 6,20. According to the International Potato Center, developing countries concentrate 95% of the production, but with low yields. Latin America produces only 1.5 million tons 8.
Viral diseases are considered a major constraint to sweet potato production worldwide 22,38,40, due to the vegetative propagation of this species and the consequent cumulative effect of virus infections 17,29. The first report of a sweet potato viral disease in Argentina was published in the 1970s. This disease, named “batata crespa”, affected cv. Criolla Amarilla and was caused by the potyvirus sweet potato vein mosaic virus (SPVMV) 30. Later, sweet potato feathery mottle virus (SPFMV) was detected in the same cultivar 31. In 1978, Argentine farmers adopted a new cultivar, Morada INTA, tolerant to both potyviruses (SPVMV and SPFMV). However, during the 1980s, this new cultivar was affected by a severe disease called sweet potato chlorotic dwarf, caused by a synergistic combination of two aphid-transmitted potyviruses (SPFMV and sweet potato mild speckling virus, SPMSV) with a whitefly-transmitted closterovirus serologically related to sweet potato chlorotic stunt virus (SPCSV) 7. Sweet potato chlorotic dwarf was successfully controlled using propagation material obtained from disease-free areas. Nevertheless, in all sweet potato-producing areas of Argentina, cv. Morada INTA has been progressively replaced by cv. Arapey INIA, an Uruguayan genotype 7.
In 2010/11, a new viral disease with severe and variable symptoms was detected in this cultivar; it was named sweet potato yellow curling disease (YC). YC causes significant yield losses, with records of up to 90% loss in experimental trials and commercial plots. In addition, YC affects the quality of the storage roots 23.
Serological tests confirmed the presence of SPFMV 4 and SPCSV (Unpublished data) in symptomatic plants. Moreover, in these plants, two pathogens that had not been described in Argentina at that time, sweet potato virus G (SPVG), a potyvirus 33 and the geminivirus, sweet potato leaf curl virus (SPLCV) 34, were detected through serological tests and PCR, respectively.
Since YC is presumed to be caused by a viral complex, this work aimed to isolate and identify the virus or viruses involved in YC disease of sweet potato and to elucidate the viral combination that reproduces YC symptomatology.
Material and methods
Source of inoculum
More than 100 plants of sweet potato cv. Arapey INIA showing chlorosis, stunting, mosaic, chlorotic rings, chlorotic patterns, blistering, distortion, reduction of foliar area, and upward leaf curling were randomly collected from 12 fields in Colonia Caroya (31°01’16.8’’ S 64°03’42.2’’ W), Colón department, Córdoba province, Argentina. Plants were transplanted to pots and maintained in the greenhouse at 25°C under controlled conditions of humidity (70-75% RH) and photoperiod (16 h light) for further analysis.
Transmission assays
Apterous aphids from a healthy colony of Myzus persicae Sulz. were reared on Raphanus sativus L. and used for transmission studies. Fasted aphids were allowed to probe briefly (one probe) on plants of sweet potato cv. Arapey INIA showing typical YC symptoms. Aphids were transferred to healthy individuals of the indicator plant Ipomoea setosa (one aphid per each one of 44 plants) and allowed to feed for 12 h; then they were killed with an aphicide (Pirimicarb) 7,13. A repetition was performed using sweet potato cv. Okinawa 100 plants infected with SPVG, SPCSV and SPLCV. The procedure was similar to the one described previously but involved 46 I. setosa plants.
To separate SPCSV from SPLCV (semi-persistent and persistent transmission, respectively), non-viruliferous Bemisia tabaci Gennadius whiteflies reared on poinsettia (Euphorbia pulcherrima Willd.), a sweet potato plant cv. Arapey infected with YC, and 42 healthy seedlings (second unfolded leaf) of I. setosa were placed in protected cages with anti-aphid mesh, at 25ºC, in a greenhouse, under controlled conditions of humidity (70-75% RH) and photoperiod (16h light). The whiteflies were removed from the cages after 1h and up to 48h of exposure to insect feeding. At 21 days after inoculation, the plants were checked for the presence of SPCSV and SPLCV by TAS-ELISA and PCR, respectively 25.
Verification of SPFMV, SPVG, SPCSV and SPLCV presence
Infection by SPFMV, SPVG and SPCSV was checked by serological tests on all inoculated plants. A local antiserum was used for SPFMV detection. The SPVGas and SPCSVas were provided by S. Fuentes (International Potato Center, Lima, Peru) and H. J. Vetten (Federal Biological Research Center, Institute of Biochemistry, Agriculture, and Forestry, Braunschweig, Germany), respectively 7,9. SPLCV was tested by PCR 34. The production of local SPVGas is discussed below.
SPVG virus purification and antiserum production
After SPVG isolation, virus particles were purified from I. setosa-infected leaves following the method described by Di Feo et al. (2000). The virus band was collected from a sucrose-CsCl step gradient (0 to 41% CsCl in borate buffer containing 20% sucrose) after ultracentrifugation (100000 x g for 5 h at 8°C), and dialyzed against 0.05 M borate buffer. Purified virus preparation of SPVG (0.02 mg/ml) was injected into a female New Zealand rabbit. Three inoculations were performed at 20-day intervals. The first inoculation (1ml of the purified virus + 2 ml of Freund’s complete adjuvant) was administered by multiple intradermal injections, whereas the other two inoculations (1 ml of the purified virus + 1 ml of incomplete Freund’s adjuvant) were administered intramuscularly. Blood sample collection started 20 days after the last injection. The titers were evaluated by Nitrocellulose membrane enzyme-linked immunosorbent assay (NCM-ELISA) 21,32, Double-antibody sandwich enzyme-linked immunosorbent assay (DAS-ELISA) 5 and Immunosorbent electron microscopy plus decoration (ISEM+D) 26.
To evaluate the optimal dilution to be used in NCM-ELISA, SPVG antiserum was serially diluted from 1:500 to 1:1024000 in Tris saline buffer + 2% skimmed milk. Samples were macerated in extraction buffer (TBS + 0.2% Na2SO3) in a 1/50 (w/v) proportion and blotted onto a nitrocellulose membrane. Positive controls were I. setosa plants infected with SPVG, sweet potato cv. Arapey INIA infected with YC and sweet potato cv. Okinawa infected with the complex (SPVG + SPCSV + SPLCV). Negative controls were healthy I. setosa and sweet potato plants. In addition, a sample of I. setosa infected with SPFMV was included to rule out the possible cross-reaction between the antiserum and this potyvirus.
For the DAS-ELISA test, IgG was purified from the SPVG antiserum. Enzyme conjugate was prepared with the purified IgG and Phosphatase Alkaline VII S (SIGMA -Aldrich) (10 mg protein/ml suspension of SO4(NH)4; 30000 enzyme units/ml). DAS-ELISA test was performed using a NUNC polystyrene plate with 96 flat-bottomed wells as support. Three dilutions of IgG (1:500, 1:1000 and 1:2000) were tested against three dilutions of enzyme conjugate (1:500. 1:1000 and 1:1500). Samples were macerated in extraction buffer (PBS + 0.05% Tween 20 + 2% PVP+ 2% skimmed milk + 0.2% SO2Na2) in a 1/10 and a 1/1000 proportion, respectively. Positive and negative controls were sweet potato plants infected with SPVG and healthy plants, respectively. Absorbance was measured using a spectrophotometer (Dynatech Laboratories, Model MRX) at 405 nm.
ISEM+D was performed according to the protocol described by Milne & Lesemann (1978). Copper grids were first covered with the SPVG-specific antiserum, diluted 1:1000 in TBS (20 mM Tris base, 500 mM NaCl, pH 7.5) and incubated for 30 min. Samples co-infected with SPVG + SPCSV were macerated in TBS containing 0.2% sodium sulfite (1/10 w/v). For decoration of virions, antiserum was diluted at 1:50 and incubated on grids for 15 min. Moreover, the modal length of virions obtained from purified preparations was determined. Observations were made under an electron microscope (JEOL JEM EX II 1220®).
Inoculation of healthy sweet potato plants with four viruses in different combinations
This experiment was designed to determine the viral combination(s) that reproduces YC in sweet potato. Scions of I. setosa plants infected individually with each of the four isolated viruses (SPFMV, SPVG, SPCSV and SPLCV) were double, triple and quadruple side-grafted onto 10 healthy plants of cv. Arapey INIA (obtained by “in vitro’’ meristem culture) and I. setosa, respectively. Six healthy plants of cv. Arapey INIA grafted with scions from YC-affected plants were used as controls.
Grafted plants were kept in protected cages with anti-aphid mesh in a greenhouse at 25°C under controlled conditions of humidity and photoperiod.
The presence of SPFMV was determined by NCM-ELISA using local antiserum 7. To detect SPCSV, a triple-antibody sandwich enzyme-linked immunosorbent assay (TAS-ELISA) was performed, as described by Gibson et al. (1998), using antisera provided by H. J. Vetten (Federal Biological Research Center, Institute of Biochemistry, Agriculture, and Forestry, Braunschweig, Germany). Infection with SPVG was confirmed by NCM-ELISA using the local antisera produced in this study. The presence of SPLCV was verified by PCR using the primers SPG1 and SPG2 designed to bind to conserved regions in open reading frames C2 and C1, and to amplify a 912-bp fragment 18.
Results
Transmission assay
Only SPFMV was transmitted to healthy I. setosa plants from sweet potato cv. Arapey INIA infected with the YC complex. However, the frequency of isolation using single aphids (M. persicae) was 77% for SPFMV and 13% for SPVG when the inoculum source was sweet potato cv. Okinawa 100 infected with SPVG, SPCSV and SPLCV. Virus sources were maintained by grafting onto I. setosa and sweet potato cv. Arapey INIA in insect-proof cages in the greenhouse.
Transmission of SPCSV and SPLCV from sweet potato plants infected with YC showed that one hour after the I. setosa seedlings were removed from the cage, 100% of the plants were infected with SPCSV and 0% with SPLCV. On the other hand, at 48 h, 100% of the plants were infected with SPLCV and 33% with SPCSV. Those plants negative for closterovirus were selected for further testing.
Virus purification and serology
SPVG was purified from single-infected I. setosa plants. The A260/A280 ratio and viral concentration of the band extracted from the CsCl gradient were 1.16 and 0.161 mg/ml, respectively. According to the NCM-ELISA test, the optimal dilution of the antiserum was 1:512000, without cross-reaction with SPFMV.
In DAS-ELISA, optimal values of A405 were obtained after 90 minutes of reaction. The most suitable dilutions of IgG and enzyme conjugate for virus diagnosis were 1:1000 and 1:500, respectively (Table 1), whereas 1/10 w/v was the most appropriate dilution of sweet potato plant tissue.
When the SPVG antiserum was used for ISEM + Decoration tests, differentially decorated virions were observed in samples of tissue infected with SPVG +SPCSV (Figure 1).
Observations were made under a transmission electron microscope (JEOL JEM EX II 1220®) (X150000). Observaciones realizadas al Microscopio electrónico de transmisión (JEOL JEM EX II 1220®) (X150000).
A modal length of 850-900 nm (150 virions) from purified suspensions was determined (Figure 2, page 112), which corresponds to the range of length established for potyviruses 37.
Inoculation
Symptoms caused by each virus combination are shown in Table 2.
The mixed infections in which SPCSV was present caused different degrees of severity.
The combination of the four viruses induced the most severe symptomatology, resembling that of YC-affected plants in the field (Figure 3): chlorosis, stunting, mosaic, blistering, leaf curling, chlorotic spotting, chlorotic patterns, reduction and distortion of leaf area, and upward curling of leaf margins.
(A) Asymptomatic leaf (healthy plant); (B) SPFMV + SPVG, feathery mottle and chlorotic spots; (C) SPFMV + SPVG + SPCSV, interveinal chlorosis, chlorotic spots and upward curling of leaf margins; (E-H) SPFMV + SPVG + SPCSV + SPLCV, feathery mottle, mosaic, vein clearing, chlorotic spots, blistering, upward curling of leaf margins, leaf area reduction and distortion. (A) Hoja asintomática (planta sana); (B) SPFMV + SPVG, moteado plumoso y punteado clorótico; (C) SPFMV + SPVG + SPCSV, clorosis internerval, punteado clorótico y curvado de hojas; (E-H) SPFMV + SPVG + SPCSV + SPLCV, moteado plumoso, mosaico, aclaramiento de nervaduras, punteado clorótico, ampollado, curvado de hojas, reducción y distorsión del área foliar.
Young plants of cv. Arapey INIA developed this symptomatology 15 days after grafting with the combination of the four viruses.
On the other hand, I. setosa became symptomatic 10 days after inoculation. Symptoms varied from mosaic, vein clearing, feathery mottling and blistering to severe leaf distortion (“shoelace”).
Discussion
Vegetative propagation is a cultural practice that facilitates efficient virus perpetuation and dissemination way between cropping seasons or growing areas 14. While several viral diseases have been reported in sweet potato, YC is the most severe one reported in Argentina so far. It is caused by at least four viruses and produces severe symptoms and significant damage in all growing areas in the country 23.
The new disease differs from the ones previously described in Argentina. Both “batata crespa” and “sweet potato chlorotic dwarf disease” affected only sweet potato plots from Santiago del Estero and Córdoba provinces. The former was caused by SPVMV, and the latter, by three viruses: SPCSV + SPFMV + SPMSV 7,30. Two viruses already present in Argentina (SPFMV and SPCSV) and two new viruses (SPVG and SPLCV) are involved in YC.
Mixed viral infections and synergistic complexes are frequent in sweet potato 36. SPFMV is the most common virus infecting sweet potato and occurs in all sweet potato growing regions 27. SPCSV interacts synergistically with SPFMV to cause sweet potato virus disease (SPVD), the most serious disease of sweet potato 1,12,19,29. The ubiquitous presence of SPFMV has often masked the presence of other viruses in sweet potato, especially those belonging to the same family, such as SPVG; thus, detecting or isolating them is very difficult 35. It is widely known that suitable management of viral diseases that affect the sweet potato crop requires rapid and accurate detection 6. However, in previous works, it has been shown that low titers of the viral agents and the high concentration of inhibitors in the sweet potato plant hinder serological and molecular diagnosis 11,14. The antiserum obtained allowed us to detect SPVG in single and mixed infections. In the latter case, the detection was evident, without cross-reaction with SPFMV, a ubiquitous virus in sweet potato crops 39. Detection reagents are available for local species involved in YC, such as SPVGas, which is used for routine diagnosis in IPAVE.
On the other hand, geminiviruses that infect sweet potato are widely distributed throughout the world. Twelve viruses belonging to the Geminiviridae family have been reported 6,15,28. They can cause significant losses in the production and quality of certain sweet potato genotypes, without noticeable symptom expression 41. SPLCV has been detected in several locations worldwide, including Taiwan, Japan, Israel, and the United States. The geographical range of this virus, however, is still mostly unknown 14. Leaf curl disease associated with SPLCV was first reported in Argentina in 2012 34. Sweet potato leaf curl Georgia virus (SPLCGV) was also reported in Argentine sweet potatoes 24. The presence of both pathogens is associated with an increase in whitefly populations 3. Therefore, it is necessary to study the dispersion of the new viral species, since climate change causes the geographical expansion of vectors such as whiteflies 2,3,10.
The global exchange of sweet potato germplasm contributes to the wide distribution of the viruses in the sweet potato production regions 19. One effective way to prevent the spread of viruses and, therefore, control viral diseases is to use virus-tested planting material.
The new disease, called yellow curling, is a serious threat to sweet potato crops in Argentina. We are conducting studies to demonstrate its detrimental effects on the production and quality of roots.
Conclusion
In this work, the first antiserum for the fast, safe and efficient diagnosis of SPVG in the country was obtained.
The four viruses involved in YC disease were isolated and identified: SPFMV, SPVG, SPCSV and SPLCV.
The interaction of SPFMV, SPVG, SPCSV and SPLCV is needed for the development of yellow curling symptoms in sweet potato in Argentina.