Document 151005
Orchids Detection, Characterization, and Management of Pineapple Mealybug Wilt-Associated Viruses John Hu University of Hawaii Pineapple in Hawaii Hawaii’s number one agricultural commodity Hawaii Agricultural Statistics Service (2002) Symptoms of MWP Healthy • • • MWP • • Reddening of the leaves Downward curling of the leaf margins Loss of turgidity, leaves reflex downwards Leaf tip dieback Plants either recover or endure further leaf tip dieback resulting in death Association of Mealybugs with the Disease Dysmicoccus brevipes (pink) Dysmicoccus neobrevipes (gray) • In 1931 Illingworth directly associated mealybugs with wilting pineapple plants • Psuedococcus brevipes: Dysmicoccus brevipes (pink) Dysmicoccus neobrevipes (gray) Association of Ants with the Disease • Caretakers of mealybugs • Protection against predators Search for the Latent Virus • • • In 1989, U.B. Gunasinghe and T.L. German isolated a closterovirus from MWPaffected pineapple Named the Pineapple mealybug wilt-associated virus (PMWaV) Based on mealybug transmissibility, placed in Ampelovirus genus Control Strategies • Amdro ®, applied as a broadcast bait (ants) • Diazinon ● Pre-plant dip (mealybugs) ● Overhead application (mealybugs) Potential Problems • Amdro® – Inactivated by moisture – Not effective against some ant species such as Technomyrmex albipes • Diazinon – Use in pre-planting dips has been eliminated Research Areas • • • • Detection Epidemiology Etiology Management Detection Assays 1. dsRNA analyses 2. EM & ISEM 3. ELISA 4. Tissue blot Immunoassay* 5. RT-PCR* Multiple Closteroviruses in Pineapple? • • 200nm ISEM revealed that not all virus particles were being decorated by monoclonal antibodies At least two serotypes exist Tissue blot immunoassay: - distinct signal - robust - minimal sample preparation - can process 100’s of samples per day PMWaV-Specific RT-PCR Assays RT-PCR Products Southern Hybridization PMWaV-1 PMWaV-2 Epidemiology 1. Virus diversity* 2. Mealybug transmission* 3. Interactions between PMWaV and other stress factors 4. Host range Multiple Closteroviruses in Pineapple? kb 23.1 9.4 6.6 4.4 2.3 2.0 M 1 2 • • A doublet of dsRNA was often resolved by agarose gel electrophoresis May represent the replicative forms of two viruses with different genome sizes Lane 1 - dsRNAs extracted from 100 g of TBIA-positive pineapple tissue 2 - dsRNAs extracted from 5 g of citrus bark infected with Citrus tristeza virus Multiple Closteroviruses in Pineapple? hsp70h Clone nt Homology • pC15 100% pC16 100% pC18 47% pC12 • • Initial cloning and sequencing revealed two distinct hsp70h genotypes in viral dsRNA PMWaV-1 PMWaV-2 PMWaV-2 Monoclonal Antibody Selection PMWaV 2 1 and 2 1 None dsRNA Analysis of PMWaV-1and PMWaV-2-Infected Plants kb 23.1 M 1 2 3 Lane 1 dsRNAs isolated from PMWaV-1-infected plants 9.4 6.6 4.4 2 dsRNAs isolated from PMWaV-2-infected plants 3 dsRNAs isolated from PMWaV-free plants Genome Organization of PMWaV-1 and PMWaV-2 PMWaV-2 HSP70 CP p20 p5 p5/6 p46/61 CPd p21 3’ RdRp 5’ P-PRO MTR HEL ? 0 ? 4 8 12 PMWaV-1 16 kb % Sequence Homology Between PMWaV-1 & -2 Gene Helicase Polymerase p5/p6 HSP70h p46/p61 Coat Protein Nucleotide Amino Acid Identity Similarity Identity 47 66 70 62 36 41 59 49 61 56 51 49 33 23 25 37 20 21 More Than Two? • • • Degenerate primers targeting conserved motifs in the Hsp70h were designed. Screening of field selections as well as pineapple accessions at the USDA-ARS pineapple germplasm repository Two clones distinct from PMWaV-1 and -2 were identified and tentatively named PMWaV-3 and -4. Sequence Homology in the Hsp70h region of PMWaVs PMWaV 1 2 3 4 1 2 3 4 38 75 88 47 37 37 67 48 76 75 39 66 - % amino acid identity % nucleotide identity PMWaV-Specific RT-PCR Assays M bp 1353 1078 872 603 310 1 2 PMWaV 3 4 - H2O 0 4 2 6 8 10 12 14 16 5’ p4 3’ p7 p21 p59 GLRaV-3 PMWaV-2 18kb p22 ? PMWaV-1 p20 p46 ? PMWaV-3 protease domain (polyprotein processing) methyltransferase domain (replication) helicase domain (replication) RNA polymerase (replication) p20 p20 p61 ? hydrophobic protein (movement) heat shock 70 homolog (structure, movement) see above (structure, movement) major coat protein (structure, movement) p61 p24 p23 p6 ? ? minor coat protein (structure, movement) see above (unknown function) see above (unknown function) see above (unknown function) Genome organization of PMWaV-1 and -3 in comparison to that of the GLRaV-3 and PMWaV-2. Boxes represent sequence domains or open reading frames (ORFs), and orthologs are colorcoordinated. +1 +2 +3 52 91 Beet yellow stunt virus (BYSV) Beet yellows virus (BYV) Genus Closterovirus (aphid transmissible) Citrus tristeza virus (CTV) 53 76 97 Sweet potato chlorotic stunt virus (SPCSV) Cucurbit yellow stunt disorder virus (CYSDV) Genus Crinivirus (whitefly transmissible) Lettuce infectious yellows virus (LIYV) 97 95 Grapevine leafroll-associated virus 3 (GLRaV-3) Pineapple mealybug wilt-associated virus 2 (PMWaV-2) Genus Ampelovirus (mealybug transmissible) Little cherry virus 2 (LChV-2) The three current genera in the family Closteroviridae are supported by vector and phylogenetic data. Dendrogram was generated using TreePuzzle 5.2 with coat protein sequence data in a maximum likelihood model. Numbers represent branch support in percentage following 10,000 puzzling steps. Genus S A L F PMWaV-2 ugc gcg uua uuuc GLRaV-3 gcu ggu ugc uuuc A G C F Q Q C V cag cag ugc guuu PMWaV-1,-3 ccg cag cgg guuu BYV P Q R V E gag gag E N aac agc S Major Coat Protein (kDa) Closterovirus 22-25 Crinivirus 28-31 Ampelovirus PMWaV-1, -3 35-38 28-29 The +1 ribosomal frameshift sequences of PMWaV-1 and -3 more closely resemble that of Beet yellows virus of the genus Closterovirus than other ampeloviruses. The major coat protein of PMWaV-1 and -3 is more similar in size to the criniviruses than the ampeloviruses. Closterovirus BYSV GLRaV-2 BYV CTV 86 LChV-1 100 Crinivirus 100 OLYaV LIYV 100 100 100 100 SPCSV 65 MVBaV CYSDV 100 100 PMWaV-2 100 68 100 PBNSPaV (p) 100 100 GLRaV-3 GLRaV-1 LChV-2 100 100 100 PMWaV-3 GLRaV-6 (p) GLRaV-9 GLRaV-5 (p) GLRaV-4 (p) PMWaV-1 Ampelovirus Phylogenetic assessment of the family Closteroviridae using full-length or partial (p) Hsp70h sequences as generated by Bayesian analysis using the BLOSUM fixed rate amino acid model. Numbers on branches are posterior probabilities and indicate branch support. LChV-1, MVBaV and OLYaV are unassigned members of the family. Viral abbreviations as in Fig. 1 or: MVBaV, Mint vein banding-associated virus; OLYaV, Olive leaf yellowing-associated virus; PBNSPaV, Plum bark necrotic stem pitting-associated virus. PMWaV-3 amino acid identity (similarity) with other PMWaVs Open reading frame Amino acid identity (similarity) Virusa RdRp Hydro HSP70 HSP70 P46 complete Coat Protein PMWaV-1 63.9 (70.6) 72.5 (82.4) 79.2 (84.7) 72.0 (78.2) 63.2 (71.5) 63.7 (70.2) PMWaV-2 30.4 (38.1) 12.8 (31.9) 44.0 (51.0) 34.9 (43.3) 21.1 (29.8) 25.8 (37.7) PMWaV-4 70.3 (70.5) Amino acid identity (similarity) of PMWaV-3 with other Ampeloviruses Open reading frame -- Amino acid identity (similarity) Virus RdRp Hydro HSP70 P46 Coat GLRaV-1 Australia 34.5 (45.4) 15.7 (23.5) 35.0 (43.0) GLRaV-3 NY1 37.6 (47.1) 25.6 (39.5) 36.6 (45.8) 20.7 (30.2) 26.0 (32.0) GLRaV-5 58.1 (67.0) 21.4 (29.9) 59.3 (70.1) GLRaV-9 CA 59.3 (67.5) 23.9 (33.6) 27.5 (33.3) LChV-2USA6b 32.2 (45.0) 16.3 (34.7) 34.2 (43.8) 19.5 (26.4) Amino acid identity and (similarity) of PMWaV-3 with other Closteroviridae members Open reading frame -- Amino acid identity (similarity) RdRp Hydro HSP70 P46 Coat Tentative Ampeloviruses GLRaV-4 CA 55.4 (65.1) 22.2 (31.1) 59.5 (67.7) 48.1 (58.8) 57.1 (67.2) GLRaV-6 CA 23.8 (33.3) 58.2 (67.4) 49.5 (59.2) 60.2 (68.8) 22.2 (50.0) 17.9 (23.4) CPd 22.6 (33.9) CP PBNSPaV 46.6 (55.2) Closterovirus GLRaV-2 Italy 34.8 (45.8) 28.5 (49.0) 33.7 (40.6) Unassigned GLRaV-7 VAA42 LChV-1 35.3 (43.9) 30.0 (42.9) 23.3 (33.3) OLYaV OLYaV Sicilian 26.0 (37.0) 30.9 (39.7) 32.6 (46.6) 22.7 (38.6) 27.3 (37.5) 27.3 (29.5) USDA National Clonal Germplasm Repository Of 35 Tested By TBIA and RT-PCR φX φX PMWaV-3 Only 12 (34%) PMWaV-1 and –3 2 (6%) PMWaV-2 and -3 4 (11%) PMWaV-1, -2, -3 2 (6%) Total 20 (57%) Pineapple mealybug wilt associated virus 1 only 2 only 3 only Selection 1 28 ± 4 1±1 0 0 0 0 Selection 2 28 ± 4 19 ± 3 0 0 0 0 Selection 3 45 ± 7 2±1 0 0 0 0 Selection 4 82 ± 5 1±1 0 0 0 0 Selection 5 99 ± 1 0 0 0 0 0 Selection 6 43 ± 7 <1 ± 1 0 0 0 0 Hybrid 4 12 ± 5 9±7 0 <1 ± 1 0 0 Hybrid 5 16 ± 10 5±4 0 5±3 2±1 0 Hybrid 6 2±2 1±1 0 2±1 0 0 Hybrid 7 <1 ± 1 <1 ± 1 0 0 0 0 Hybrid 8 0 0 0 0 0 0 Hybrid 9 31 ± 7 5±2 9±1 3±3 5±1 5±1 Clone 1 and 3 2 and 3 1, 2, and 3 PMWaV incidence, Hybrid 1, Oahu island PMWaV incidence (Mean ± S.E. ) Source Loc Costa Rica Mean +1 +2 +3 1&2 2& 3 1&3 1,2,3 1 42±8 17±11 18 2±4 8±6 3±4 2±2 2 31±10 16±5 3 4±3 5±6 3±4 0±2 36 ±10 16±10 10 3 ±4 6±6 3 ±4 1 ±2 What is the role of the pineapple mealybugs in PMWaV dissemination Dysmicoccus brevipes D. neobrevipes Transmission of PMWaV No. of PMWaV infected plants/ total no. exposed Experimental Initial Days after initial mealybug introduction Conditions status 44 75 125 175 ________________________________________________________ Without mealybugs PMWaV “-” 0/40 0/40 0/40 0/40 0/40 PMWaV “+” 20/20 20/20 20/20 20/20 20/20 Virus-free mealybugs PMWaV “-” 0/40 0/40 0/40 0/40 0/40 Viruliferous mealybugs PMWaV “-” 0/40 7/40 21/40 31/40 40/40 PMWaV “+” 20/20 20/20 20/20 20/20 20/20 Effect of Mealybug Densities # of PMWaV infected plants/ total # exposed Days after Number of “crawlers” introduction 1 5 10 20 40 _____________________________________________ 20 0/45 0/15 1/15 2/15 5/15 30 0/45 1/15 6/14 7/15 8/15 50 1/45 3/15 10/14 14/15 13/15 75 2/45 3/15 10/14 15/15 14/15 Effect of Mealybug Age # of PMWaV infected plants/ total # exposed Days Prelarvaposition period Larvaposition Postafter 1st 2nd 3rd young old larvapos. feeding gravid gravid nonfeed. ___________________________________________________ 30 1/20 7/20 13/20 2/20 1/20 0/15 55 5/20 11/20 16/20 7/20 1/20 0/15 80 6/20 15/20 20/20 8/20 1/20 0/15 Virus Transmission • • • • PMWaV 1 and 2 can be transmitted by mealybugs. 1 mealybug can cause transmission; 20 mealybugs/plant = 100% transmission. 1 month after transmission, virus infection can be detected by tissue blotting. Instars are better vectors than adults. Etiology 1. Symptom induction 2. Mealybug transmission of PMWaVs* Symptom Induction Mealybugs PMWaV + - + no MWP no MWP no MWP YES ! Mealybug-free PMWaVPMWaV free infected Mealybug-inoculated PMWaVPMWaVfree infected MWP Susceptibility Pineapple Selection 1 Selection 2 Selection 3 Selection 4 Selection 5 X/X 0/10 0/10 0/10 0/10 0/10 V/X 0/10 0/10 0/10 0/10 0/10 V/M 17/20 20/20 18/20 18/20 10/10 Transmission of PMWaVs and Symptom Induction Mealybugs D. brevipes D. neobrevipes D. brevipes D. neobrevipes D. brevipes D. neobrevipes Acquisition Source PMWaV-2 PMWaV-2 PMWaV-1 PMWaV-1 PMWaV-free PMWaV-free No. infected/ MWP No. exposed 54/72 20/20 28/30 20/20 7/10 0/10 10/10 0/10 0/10 0/10 0/10 0/10 Vector Transmission and MWP Acquisition source Virus combination Infection incidence Symptom incidence S2 H5 S2 HY5 D. brevipes Accession 100 1 and 3 4/5 5/5 0/5 0/5 Accession 111 2 and 3 4/5 5/5 4/5 5/5 Accession 126 Hybrid 9 Selection 1 2 and 3 3 - 3/5 4/5 0/5 4/5 5/5 0/5 3/5 0/5 0/5 4/5 0/5 0/5 D. neobrevipes Accession 100 1 and 3 5/5 5/5 0/5 0/5 Accession 111 2 and 3 5/5 5/5 5/5 5/5 Accession 126 2 and 3 5/5 5/5 5/5 5/5 Hybrid 9 3 5/5 5/5 0/5 0/5 Selection 1 - 0/5 0/5 0/5 0/5 PMWaV-3 can be acquired and transmitted by pink and grey pineapple mealybugs. Dysm icoccus brevipes D. neobrevipes Plants infected with PMWaV-3 and exposed to mealybugs did not develop MWP. Back row: ‘Smooth Cayenne’ infected with PMWaV-3 only Front row: Hybrid 9 infected with PMWaV-3 only All plants were exposed to Dysmicoccus brevipes Left: Plants infected with PMWaV-3 only that were exposed to Dymiscoccus brevipes Right: Plants infected with PMWaV-3 and PMWaV-2 that were exposed to Dymiscoccus brevipes Working Hypothesis of the Etiology of MWP Pineapple plants have developed tolerance to infection by PMWaVs and do not develop wilt symptoms when infected by PMWaVs. When mealybugs feed on these plants, the insects inject an agent that suppresses this tolerance. As a result, MWP symptoms develop. This hypothesis also explains the recovery phenomenon: if the mealybug factor is removed, plants regain tolerance to PMWaV infection and MWP symptoms disappear. BADNAVIRUSES •Family Caulimoviridae Genus Badnavirus • Circular dsDNA (7.35 kb – 8.3 kb) • Possible synergistic effects with other viruses Host plants : MWP DISEASE COMPLEX Vector PMWaV-2 + Mealybug feeding PMWaV-2 Synergistic? Badnavirus MWP PCR with degenerate oligonucleotide Badna1a & Badna 4 using total DNA from pineapple plants representing different hybrids. Expected target size = 600 bp Products were cloned and sequenced. Many products are similar to retro-like elements such as dea1, gypsy. gag, etc. Several were similar to badnavirus sequences. Neighbor joining using PAUP. Based on 200 amino acids Optimized alignment using ClustalX. Badnavirus Detection Polymerase chain reaction assays (PCR) • Nucleic acid extraction (DNeasy® kit) Badnavirus Primer sets Amplicon size A B C M 500 A 642/573 505 bp B 654/655 553 bp C 656/657 563 bp M 652/653 573 bp Agarose gel analysis Purify, purify, purify………………………………. 100 nm 100 nm 100 nm Badnavirus incidence Source No. of plants sampled Badnavirus incidence (Mean percentage) +A +B +C +M Hybrid 1 (Costa Rica) 30 0 100 100 47 Hybrid 1 (Philippines) 30 0 100 100 23 12 100 100 100 100 12 10 100 100 100 12 50 100 100 100 Hybrid 2 Hybrid 2 Hybrid 3 Objective 1. Develop universal and specific polymerase chain reaction assays to detect, differentiate, and determine the distribution of badnaviruses in pineapple and other potential host plants Identification of badna-like viruses Detection of integrated viral sequences Development of reliable specific and universal detection assays Objective 2. Evaluate the roles of PMWaVs, PBVs, and mealybugs in the etiology of MWP Vector transmissibility MWP etiological studies Functional assays used to identify suppressors of RNA Transient expression assays A. Assay for suppressors of local silencing B. Assay for suppressors of systemic silencing silencing Identification of p20 as suppressor of RNA silencing by the Agrobacterium coinfiltration assay. Leaves of the 16c GFP plants were infiltrated with an A. tumefaciens EHA105 carrying GFP together with an A. tumefaciens EHA105 carrying the empty binary plasmid GFP:-- (left), GFP:TBSVp19(middle) and GFP: PMWaV-II (right); The green fluorescence images of the coinfiltrated leaves were taken 13 days postinfiltration under a long-wave UV lamp. Strategies for Reducing the Incidence of PMWaVs and MWP 1. Use virus-free planting material 2. Use physical-based methodologies (ie. “edge quarantines”, roguing, planting bed spacing, etc.) 3. Develop a system that can predict when mealybug control should be instigated 4. Compare and demonstrate IPM tactics 5. Develop PMWaV-resistant transgenic pineapple Strategy 1. Use PMWaV-free Pineapple Material for MWP Management 1. Screen propagation material with antibodies in tissue blot immunoassays before or after tissue culture propagation (hybrids) 2. Virus elimination by meristem tissue culture Removal of apical meristem Resulting plant 5122 plants were gouged 7 slips per plant 36,000 propagules Strategy 2. Use Physical-based Methodologies to Reduce PMWaVs and MWP in the Field 1. Selection of initial planting area 2. Spatially-based quarantines for selection of planting material 3. Manipulation of planting bed spacing 4. Roguing of PMWaV-infected plants Strategy 3. Develop a system that can predict when mealybug control should be Instigated 1. Develop a quantitative mealybug detection system 2. Monitor PMWaVs and MWP incidences over time Determine if correlations exist between relative mealybug numbers detected and virus spread and mealybug wilt Strategy 4. Compare and demonstrate IPM tactics Based on alternative technologies including: 1. Virus incidence 2. Pesticide application methods 3. Pesticide application timing The purpose is to reduce the use of the more toxic pesticides! Strategy 5. Develop PMWaV-resistant Transgenic Pineapple Plants 1. Develop inverted repeat gene constructs 2. Optimize transformation and regeneration systems 3. Screen resistant plants Goal Application of RNA-mediated virus resistance to this pathosystem will allow for the development of pineapple plants which are resistant to PMWaV and MWP. Gene Constructs pBI121 Backbone RB 1 2 NOS NOS NPT II NPT II NOS-T NOS-T UBI9 UBI9 AMV AMV LB CPS NOS-T CPS HSP CPAS NOS-T pCAMBIA1300 Backbone 3 UBI9 AMV 4 UBI9 AMV CPS NOS-T 35S CPS HSP CPAS NOS-T HYG 35S 35S HYG 35S Pineapple Transformation and Regeneration Systems Conclusions 1. There are at least three distinct PMWaVs. Specific and sensitive assays have been developed for detection of these viruses. 2. PMWaVs are transmitted by mealybugs. 3. PMWaV-2 and another factor associated with mealybug feeding result in mealybug wilt of pineapple. 4. PMWaV-2, but not PMWaV-1 and PMWaV-3, plays an essential role in the etiology of MWP. Conclusions 5. Badnaviruses are being characterized; PCR assays are being developed. 6. Gene silencing suppressors are being identified and used to study the potential involvement in symptom development. 7. Strategies are being evaluated for control of MWP, including PMWaV-resistant trangenic pineapple plants. Acknowledgments D. Sether, E. Perez, M. Melzer, H.Ma, V. Subere, L. Martinez, K, Cheah A. Karasev, C. Nagai, F. Zee, B. Sipes P. Wood, C. Hubbard, C. Oda, H. Fleisch Acknowledgments USDA-ARS USDA-CSREES Hawaii Department of Agriculture Pineapple Growers Association of Hawaii Banana bunchy top virus (BBTV) is the most important virus disease in banana worldwide. Kheng Cheah, Chen Yan Eden Perez Impacts 1. BBTV-resistant banana plants 2. Resistance to other banana diseases 3. Improved quality of bananas 4. Vaccines for oral immunization Citrus tristeza in Hawaii • • Citrus tristeza closterovirus (CTV), the causal agent of citrus decline and stempitting, was first reported in Hawaii in 1952 Brown citrus aphid (Toxoptera citricidus), the most efficient vector of CTV, has been present in Hawaii since 1907 Mike Melzer Ph.D. student Stem-pitting Impacts • Help to develop a new citrus industry in Hawaii. • Our research will benefit the entire citrus industry of the USA.
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