Releases in israel ofAphelinus perpallidus,a recently introduced parasite of the pecan blackmargined aphid,Monellia caryella

Six shipments totaling 3452 mummies of the blackmargined aphid,Monellia caryella (Fitch), parasitized withAphelinus perpallidus Gahan, were obtained by air freight during the years 1982-1985 from Texas A&M Research Center, El Paso, Texas. About two-thirds of the mummies did not yield parasites. A colony ofA. perpallidus was established in the laboratory. Under laboratory conditions the percentage of emerged parasites was higher than that in the imported mummies, and the parasite had very limited impact on the aphid population. Field releases of the parasite were made but no establishment ofA. perpallidus was observed through the years.     

Arthropod fauna and main insect pests of plane trees in Israel

Fifty-four insect and four mite species are included in a list of the entomofauna of plane trees in Israel. Only two species are monophagous:Phyllonorycter platani (Stgr.) (Lepidoptera: Gracillariidae) andEdwardsiana iranicola Zachv. (Heteroptera: Cicadellidae). Four species are noxious:P. platani, the main insect pest of the plane trees in Israel;Zeuzera pyrina L. (Lepidoptera: Cossidae);Kalotermes flavicollis F. (Isoptera: Kalotermitidae); andE. iranicola. Of much lesser importance areTargionia vitis Sign. (Homoptera: Diaspididae),Heliothrips haemorrhoidalis Bché. andRetithrips syriacus May. (Thysanoptera: Thripidae). About half of the listed species are natural enemies and many are parasites ofP. platani. Details are given on the noxious species, together with recommendations for prevention and control.     

The overwintering mode ofBemisia tabaci and its parasitoids in Israel

Wild and cultivated plants in the vicinity of Kibbutz Nahshon and a few additional locations in Israel were sampled for the presence ofBemisia tabaci Genna-dius (Homoptera: Aleyrodidae). The whiteflies, together with their parasites,Eretmocerus mundus andEncarsia lutea, were found to develop on numerous host species throughout the winter. Especially high levels were reached onLan-tana camara, Abutilon grandifolium andIpomoea batatas. During late winter and spring the population on these hosts declined. From April onwards the populations increased on potatoes and sunflowers.     

Introductions of beneficial insects into Israel by the Institute of Plant Protection Quarantine Laboratory,ARO, during 1971-1978

A list is given of the beneficial insects introduced into Israel during 1971–1978 by the Institute of Plant Protection Quarantine Laboratory for biological control of plant pests. The list includes 15 species of Hymenoptera (14 parasites and one parasite/predator) as well as four coleopterous predators. Included are each shipment’s origin, date and sender, as well as the results of these introductions.     

The Mediterranean vine mealybug and its natural enemies in southern Israel

The phenology of the Mediterranean vine mealybug population in the vineyards of southern Israel was found to be characterized by a peak, occurring between mid-May and mid-June, followed by a sharp drop during July. A second, smaller peak occurs between October and December. During winter the mealybugs remain beneath the bark of the trunk at a very low population level. The primary parasites, all of the anagyrine Encyrtidae, were (in descending order of abundance):Anagyrus pseudococci, Leptomastix flavus, Clausenia josefi, Pauridia peregrina, andLeptomastidea abnormis. The hyperparasites wereAchrysopophagus aegyptiacus (Encyrtidae) andPachyneuron siculum (Pteromalidae).Tetrastychus sp. (Eulophidae) andThysanus sp. (Signiphoridae), very rare parasites, remained unclassified.Hyperaspis spp. andScymnus spp. (Coccinellidae) are mealybug predators. They were sometimes parasitized byHomalotylus quaylei (Encyrtidae). The phenology of the entomophagous insects is described.     

Braconidae (Hymenoptera) associated with forest and ornamental trees and shrubs in Israel

Data are presented on the occurrence of Braconidae (Hymenoptera parasitica) parasitizing insects associated with forest and ornamental trees and shrubs in Israel. Fifty-five genera of plants are listed, the richest in braconid fauna being tamarisk (9 species); acacia, pistachio and poplar (8 species each); carob and oak (7 species each). Of the 95 species of insect hosts mentioned, 53 are Lepidoptera, mostly Gelechiidae (7 species), Pyralidae (6 species), Noctuidae (5 species), Gracillariidae, Tortricidae, Geometridae, Lymantriidae and Lycaenidae (3 species each); 44 are Coleoptera, mostly Cerambycidae (13 species), Scolytidae (12 species), and Bostrichidae (9 species); three are Diptera. Of the 92 species of braconids listed, of which only 65 have been fully named, 56 develop in Lepidoptera, mostly Noctuidae (15 species), Gelechiidae (11 species) and Pyralidae (9 species); 33 species develop in Coleoptera, mostly Cerambycidae (12 species, Bostrichidae (10 species) and Scolytidae (5 species); and three species develop in Diptera. Thirty-eight species are new to the fauna of Israel; at least three of them are new to science,viz., Gnaptodon, Gildoria andDendrosotinus titubatus Papp.     

Control of phytophthora leaf blight of taro (Colocasia esculenta) by fungicides and roguing

Six fungicides were evaluated under laboratory and field conditions for control of Phytophthora leaf blight of taro,Coloeasia esculenta, incited byPhytophthora colocasiae. Inin vitro tests Deraosan 65W was the most effective in inhibiting the mycelial growth of the test pathogen followed by Difolatan 80W, Fytolan (copper oxychloride), Apron 35F, Topsin-M 50W and Dithane Z-78 75W. Excellent control was obtained with Demosan 65W and Difolatan 80W, good control with Apron 35F, fair control with Fytolan, and poor control with Topsin-M 50W and Dithane Z-78 75W. Results ofin vivo tests were correlated with those of thein vitro tests. Roguing of infected leaves did not eradicate the pathogen but can only delay epiphytotics.     

Plant ferredoxin-like protein enhances resistance to bacterial soft rot disease through PAMP-triggered immunity in Arabidopsis thaliana

The protection of plants against bacterial disease is one of the important issues that need to be studied in agricultural applications. The application of a transgene, such as a gene that encodes plant ferredoxin-like protein (PFLP), to generate resistant plants is one possible strategy. Our previous reports have demonstrated that transgenic plants that express extracellular PFLP (ESF plants) are more resistant to bacterial pathogens. This protein intensifies the hypersensitive response (HR) in plants when they are infiltrated by a pathogen-associated molecular pattern (PAMP), harpin (HrpZ), from Pseudomonas syringae. In addition, this intensified HR is associated with the expression of membrane-bound NADPH oxidase. Thus, we attempted to determine the involvement of PFLP in intensifying PAMP-triggered immunity (PTI) to enhance disease resistance. First, we showed that transgenic Arabidopsis plants with the pflp gene were resistant to bacterial soft rot caused by Pectobacterium carotovorum subsp. carotovorum (Pcc). Then, the fliC gene which encoded flagellin from Pcc was cloned and expressed. The FliC protein was used in the functional study with PFLP in Arabidopsis Col-0 plants. The reactive oxygen species (ROS) generation and HR ratio were induced by the treatment with both PFLP and FliC together, but they were not induced by treatment with PFLP or FliC alone. Similar results were confirmed in ESF plants, where FliC elicited rapid ROS accumulation and callose deposition. Moreover, we demonstrated that the PFLP-intensified ROS generation and HR were related to Ca²⁺ influx and activation of NADPH oxidase. We concluded that the PFLP-intensified disease resistance is associated with the intensification of PAMP-triggered immunity.     

Sensitive detection of two plant viruses by enzyme-amplified elisa

Enzyme-amplified ELISA (enzyme-linked immunosorbent assay) increased the sensitivity of detection of citrus tristeza virus and papaya ringspot virus in plant sap by 25- and 125-fold, respectively, compared with direct double antibody sandwich ELISA. The advantages of the new substrate system for the detection of low concentrations of viruses in plants are discussed.     

Development of conventional and real-time PCR protocols for specific and sensitive detection of Colletotrichum capsici in chilli (Capsicum annuum L.)

Anthracnose, caused by Colletotrichum capsici, is a major disease of chilli (Capsicum annuum L.) affecting both fruit and seed quality. The pathogen is both internally and externally seedborne. However, a rapid and sensitive method for detection of this pathogen in seeds is currently limited. In this study, a polymerase chain reaction (PCR) method based on sequence characterized amplified region (SCAR) marker was developed for specific and sensitive detection of C. capsici in chilli seeds and fruits. The developed SCAR primers were highly specific to C. capsici and resulted in the amplification of an expected 250-bp fragment from genomic DNA of all seven of the C. capsici isolates tested. No amplification occurred when the SCAR primers were tested with genomic DNA from three other fungal isolates and four other Colletotrichum species. The SCAR primers successfully amplified similar sized fragments from DNA derived from C. capsici-infected chilli fruits. The molecular detection sensitivity of C. capsici was 1 pg of purified C. capsici DNA template and 25 ng of DNA from C. capsici-infected chilli fruits. A real-time PCR assay was also developed using SYBR Green chemistry for detection of C. capsici in chilli fruits and seeds. The standard curve obtained showed a linear correlation between copy number of the cloned target DNA sequence of C. capsici and cycle threshold (Ct) values, with R² of 0.98. These PCR-based assays may be highly useful in detection of this important pathogen in chilli seeds and fruits in plant quarantine laboratories.     

Phenotypic and genotypic structure of Phytophthora infestans populations on tomato and potato in the North of Thailand in 2000–2002

A total of 80 single–lesion isolates of Phytophthora infestans were collected from tomatoes and potatoes in several locations in Chiang Mai and Tak provinces in 2000–2002. These isolates were analyzed for mating type, metalaxyl sensitivity, mitochondrial DNA (mtDNA) haplotype RFLP pattern as determined by probe RG57, and for microsatellite markers. All isolates were A1 mating type. Isolates from tomato were usually sensitive to metalaxyl, but isolates from potato were usually resistant to metalaxyl. With one exception, all tomato isolates were related to the US-1 clonal lineage. With two exceptions, all potato isolates were related to two European lineages. In these two provinces, the populations of P. infestans on tomatoes are clearly different from those on potatoes.     

Alien scale insects (Hemiptera Coccoidea) in European and Mediterranean countries: the fate of new and old introductions

This contribution focuses on recent interceptions and introductions of alien scale insects and their current distribution in European and Mediterranean countries. Data and collections were gathered in markets, nurseries, and botanical gardens, mostly in Italy, either indoors or outdoors. New or recent records of the following alien species are presented: Exallomochlus hispidus (Morrison); Ferrisia virgata (Cockerell) (Pseudococcidae); Coccus viridis (Green); Milviscutulus mangiferae (Green) (Coccidae); Aonidiella orientalis (Newstead); Aspidiotus destructor Signoret; Aulacaspis tubercularis Newstead; Fiorinia fioriniae Targioni Tozzetti; Lepidosaphes pinnaeformis (Bouché); Pseudaulacaspis brimblecombei Williams (Diaspididae). New data and pest status of Phoenicococcus marlatti Cockerell (Phoenicococcidae) and Trabutina mannipara (Hemprich & Ehrenberg) (Pseudococcidae) are also reported. The possible repeated introductions of the latter from North Africa to south Italy by trans-Mediterranean winds, is hypothesized.     

Analysis of genetic and virulence variability of Stemphylium lycopersici associated with leaf spot of vegetable crops

Stemphylium lycopersici (Enjoji) W. Yamam was initially described from tomato and has been reported to infect different hosts worldwide. Sequence analyses of the internal transcribed spacer (ITS) regions 1 and 2, including 5.8S rDNA (ITS-5.8S rDNA) and glyceraldehyde-3-phosphate dehydrogenase (gpd) gene, random amplified polymorphic DNA (RAPD) and inter-simple sequence repeat (ISSR), as well as virulence studies were conducted to analyze 46?S. lycopersici isolates. Stemphylium lycopersici isolates used in this study were obtained from diseased tomato (Solanum lycopersicum L.), eggplant (Solanum melongena L.), pepper (Capsicum annuum L.) and lettuce (Lactuca sativa L.) from major vegetable growing regions of Malaysia, including the three states of Pahang, Johor and Selangor between 2011 and 2012. Phylogenetic analysis of a combined dataset of the ITS-5.8S rDNA and gpd regions indicated that all isolates were clustered in the sub-cluster that comprised S. lycopersici, and were distinguished from other Stemphylium species. Cluster analyses using the UPGMA method for both RAPD and ISSR markers grouped S. lycopersici isolates into three main clusters with similarity index values of 67 and 68 %. The genetic diversity data confirmed that isolates of S. lycopersici are in concordance to host plants, and not geographical origin of the isolates. All S. lycopersici isolates were pathogenic on their original host plants and showed leaf spot symptoms; however, virulence variability was observed among the isolates. In cross-inoculation assays, the representative isolates were able to cause leaf spot symptoms on eggplant, pepper, lettuce and tomato, but not on cabbage.     

Evaluation of biochemical methods for the diagnosis of the avocado sunblotch viroid in Israel

The reliability of biochemical diagnostic methods for avocado sunblotch viroid (ASBV) was evaluated for the Israeli avocado propagation program. Polyacry-lamide gel electrophoresis (PAGE) was compared with hybridization toin vitro ³²P-labeled cDNA and ASBV-RNA probes. Although hybridization to a cDNA probe was the most sensitive method, not all known infected plants were detected. In the light of these results, the problem of diagnosing ASBV in the Israeli propagation program is discussed.     

Detection and estimation of Citrus Tristeza Virus infection rates based on Elisa Assays of packing house fruit samples

Enzyme-linked immunosorbent assay (ELISA) proved to be a sensitive detector for citrus tristeza virus (CTV) in orange fruits (Citrus sinensis (L.) Osbeck). Samples of five fruits were taken from 350-kg packing house containers and tested by ELISA to predict the infection rate of CTV in two infected orange groves. The predicted infection rates, 1% and 11%, were in reasonable agreement with the observed rates of 1% (15/1400) and 16% (324/2053), respectively. The 360 test samples from reputedly uninfected groves all tested negative. These results suggest that the ELISA procedure may provide a general method of detecting viral or other systemic pathogenic infections using the fruit as the test material in place of tree tissue. Fruit samples can be collected routinely at the packing house to reduce test costs.     

Enzyme-linked immunosorbent assay (ELISA) for the detection of potato viruses A and Y in potato leaves and sprouts

With the enzyme-linked immunosorbent assay (ELISA) potato virus A (PVA) could be detected reliably in potato sprouts, especially when these were young and sappy. The detection of this virus in leaves of glasshouse-grown potato plants was less reliable. The tobacco veinal necrosis strain of potato virus Y (PVY^N) was readily demonstrated in foliage of glass-house-grown potato plants using an antiserum to this strain. Plants infected with the common strain (PVY^O) did not react in ELISA with this antiserum. In young sappy sprouts, using the PVY^N antiserum, PVY^N could be detected reliably when samples with PVY^O were excluded, as the reaction of samples infected with the latter virus was intermediate between PVY^N-diseased and PVY-free samples. PVY was also detected in plants inadvertently infected during the experiments.     

Detection and partial molecular characterization of Plum pox virus on almond trees in Turkey

Almond (Prunus dulcis) is one of the well known stone fruit species grown for its unripe fruits and delicious seeds in Turkey. In the Trakya region, however, some prevailing virus infections have reduced almond yields and quality. In ten districts of Trakya, 260 leaf samples were collected from affected almond trees in June 2010. DAS–ELISA assays and RT-PCR tests were employed for the identification of viruses. As a result of these detection studies, five of the 260 leaf samples gathered from symptomatic almond trees had Plum pox virus (PPV), 81 of them had Prunus necrotic ringspot virus (PNRSV), and 11 samples contained Prune dwarf virus (PDV). Only four out of 260 samples had a mixture of these viruses. Partial nucleotide sequences of five almond isolates of PPV were determined and compared with 17 other PPV isolates in databases. Computer analysis of obtained and published nucleotide sequences showed identity ranged from 75.72% to 96.87%. Of the five PPV almond isolates obtained, however, there was a close nucleotide identity of 95.82–96.61% to Turkish isolates. Phylogenetic analysis of nucleotides and amino acids showed that five PPV isolates of almond from the Trakya Region of Turkey were clustered in the same subgroup with PPV-T Turkish isolates in GenBank. Therefore we can consider almond isolates of PPV as PPV-T strain, like the two other isolates from apricot trees in Turkey.     

Pyrethroid synergism and prevention of emergence inTribolium castaneum andMusca domestica vicina by the insect growth regulator RO 13-5223

Ethyl [2-(4-phenoxyphenoxy)ethyl] carbamate (RO 13-5223) at a dietary concentration of 100 mg kg^-1 synergized the toxicity of thetrans- andcis-isomers of permethrin and cypermethrin in inhibiting the growth (measured as gain in larval weight) ofTribolium castaneum andMusca domestica vicina. With both species the synergism factor forcis-cypermethrin with 100 mg kg^-1 synergist was 1.5- to twofold for RO 13-5223 and about fourfold for piperonyl butoxide. Synergism was more pronounced with first instar than with fourth instarT. castaneum larvae. Methoprene was not a pyrethroid synergist withT. castaneum larvae, so the synergistic effect of RO 13-5223 appears to depend on its structural features and not its insect-growth-regulator activity. Joint application of RO 13-5223 and pyrethroids resulted in a dual effect on bothT. castaneum andM. domestica: increased inhibition of larval growth due to pyrethroid synergism, and progeny suppression — expressed by larval and pupal mortality — due to RO 13-5223 juvenilizing activity.     

Involvement of Phytophthora cryptogea in sweet cherry decline in Turkey

Sweet cherry is a major commercial crop in Turkey, the most important producer of the fruit worldwide. Sweet cherry decline was observed in an orchard in Ankara province of Turkey. Affected young trees exhibited reduced tree vigor, yellowing and wilting of leaves, and dieback symptoms resulted in tree death. A Phytophthora sp. was consistently isolated from necroses that appeared on taproots and crowns. The pathogen was identified as Phytophthora cryptogea based on several morphological features and DNA sequence of the internal transcribed spacer (ITS) region. P. cryptogea was pathogenic on excised shoots and 1-year-old cherry rootstocks. This is the first report of P. cryptogea causing disease of sweet cherry in Turkey.     

Identification and species status of the mango biotype of Colletotrichum gloeosporioides in Ghana

Research work was carried out to identify and ascertain the species status of the mango biotype of Colletotrichum gloeosporioides infecting mangoes in Ghana. Forty five isolates of Colletotrichum species were collected from 12 districts in Ghana while five each were obtained from mango fruits from Florida, Mexico and Puerto Rico. The entire internal transcribed spacer region, partial beta-tubulin gene and partial glyceraldehyde-3-phosphate dehydrogenase gene of isolates were sequenced and used in phylogenetic studies. The results of the sequence analysis of the first ribosomal transcribed spacer (ITS 1) region showed that 35 % of the isolates from Ghana and all the five isolates from Mexico were the mango biotype of C. gloeosporioides, while the others were not. Phylogenetic studies showed that the mango biotype of the pathogen was Colletotrichum asianum but not C. gloeosporioides as previously thought. However, the other isolates that were not the mango biotype were identified as Colletotrichum siamense and Colletotrichum species which had probably cross-infected mango from other fruit crops in the field.