Middle East Journal of Applied Sciences 3(3): 105-112, 2013 ISSN 2077-4613 Soil solarization for controlling soil borne fungi of Tomato (Lycopersicon esculentum Mill.) plants. 1: Effect of hot water treatment and exposures time on Viability of tomato soil borne pathogenic fungi
Riad S.R. El–Mohamedy and Farid Abd- El-Kareem
Plant Pathology Department, National Research Center, Dokki, Giza, Egypt
ABSTRACT
Viability of tomato soilborne Pathogenic fungi i.e, F. oxysporum f. sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici( FORL), F.solani, R. solani and S. rolfsii were tested against different temperatures and exposure times in digital water path under laboratory conditions. The lethal temperatures to R. solani, F. solani and S. rolfsii when were exposed to temperatures for one minutes as agar disks and/or growth suspension were 54.0, 58.0,56oC and 52.0, 56.0 or 54.0oC respectively. Meanwhile, the lethal temperatures to F. oxysporum f. sp. lycopersici (FOL)and F. oxysporum f.sp. radicis lycopersici(FORL)were 56 C and 54oC when were exposed to temperatures for one minutes as agar disks or growth suspension respectively. Chlamydospores are more resistant to high temperatures as they were killed at 62 and 60oCfor F. solani and FOL or FORL respectively.While Sclerotia were killed at 58.0 C for R. solani and S. rolfsii when exposed to hot water for one minute. Sub lethal temperatures reduced the linear growth of F. solani, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici (FORL) more than 50% and significantly reduced all resting stage production of F. solani ,F.oxysporum f.sp. lycopersici(FOL), F. oxysporum f.sp. radicis lycopersici (FORL), R. solani and S. rolfsii. Under greenhouse conditions results indicated that sublethal temperatures significantly reduced the root rot and wilt diseases for all tested fungi. It could be suggested that lethal or subletal temperatures resulted from soil solarization could be effectiveness in management tomato soilborn pathogenic fungi. Key word: Tomato- soilborne fungi -lethal temperatures-heat treatment. Introduction
Tomato (Lycopersicon esculentum Mill.) plants are the one of most important vegetable crops in Egypt and
other countries. Rhizoctonia solani, Fusarium solani, Fusarium oxysporum f.sp. lycopersici ( FOL), Fusarium oxysporum f.sp. radicis lycopersici( FORL) ,and Sclerotium rolfsii are the most damaging soil-borne diseases of tomato and becoming more common in greenhouse tomato production. The disease occurs in both the greenhouse and the field on tomato worldwide and causes significant losses in tomato production (Gotta and Tameitti , 1990 ; Dwivedi 1991; Rattink ,1993; McGovern et al., 1998; Kuckareck et al., 2000).
Soil solarization was carried out as transparent polyethylene plastic placed on moist soil during the hot
summer months increases soil temperatures to levels lethal to many soil-borne plant pathogens, weeds and nematodes ( Primo and Cartia, 2001; Abd-El-Kareem, et al., 2004; Culman, et al., 2006, Farag and Fotouh, 2010 and Saied, 2011). Solarization also effectively controls weeds, increases soil nutrient availability (Schreiner, et al., 2001) and increases populations of known beneficial bacteria and fungi (Kaewruang, et al., 1989; Gamliel and Katan, 1991 and Abdel-Kader and Ashour, 1999). Heating the surface soil over a period of several weeks helps to control pathogenic fungi and lead to reduction of plant diseases caused by soil borne fungi (Abd-El-Kareem, et al., 2004; Culman, et al, 2006 and Farag and Fotouh, 2010). The present work was designed to study the effect of hot water temperatures and exposures time on viability of tomato soil borne fungi under laboratory and green house conditions.
Materials And Methods Effect of hot water treatment on viability of tomato soilborne fungi: Viability of agar disks with mycelia, growth suspension and resting stages of Rhizoctonia solani, Fusarium solani, Fusarium oxysporum f.sp. lycopersici ( FOL), Fusarium oxysporum f.sp. radicis lycopersici (FORL), and Sclerotium rolfsii was carried out according to the method described by Whiting, et al., (2001). Growth agar disks, growth suspension and resting stage of tomato soil borne fungi were evaluated at different
Corresponding Author: Riad S.R. El–Mohamedy, Plant Pathology Department, National Research Center, Dokki, Giza, Middle East j. Appl. Sci., 3(3): 105-112, 2013
temperatures and exposure times using digital hot water bath (Neslab GP-300 Series Constant Temperature Bath, Union City, CA). Screw-cap glass vials, 20 cm long and 20 mm in diameter, containing 20.0 ml sterilized water were placed in water path at different temperatures.
Effect of hot-water treatment on mycelia agar disks viability of tomato soilborne fungi: Disk of agar with mycelia and spores 6- mm diameter were cut from the grown edge of 10 days -old
cultures of R.Salami; F. solani ; S. rolfsii; F. oxysporum f.sp. lycopersici (FOL); F. oxysporum f.sp. radicis lycopersici (FORL) growing on PDA medium. Agar disks were transferred to Screw-cap glass vials, 20 cm long and 20 mm in diameter, containing 20.0 ml sterilized water placed in water path at 25, 50, 52, 54, 56, and 58 oC for different exposures time i. e. 1, 10, 20, and 30 minutes. Treated growth agar disks were dried using sterilized filter paper and transferred into Petri-plates containing PDA medium. Five Screw-cap glass vials , and 3 disks per each were used for each treatment .Viability of mycelia from agar disk that had been subjected to previous temperatures with different exposure times was assessed by planting treated disks on PDA medium and incubated at 25 ºC for 5 days .Disks that showing growth or non- growth were recorded. Effect of hot-water treatment on growth suspension viability of tomato soilborne fungi: Plates with growing colonies of R. solan; F. solani; S. rolfsii; F. oxysporum f.sp. lycopersici (FOL) and F. oxysporum f.sp. radicis lycopersici (FORL) grown on PDA medium were flooded with 10 ml of sterile water and mycelia or spores were released using a sterile inoculation loop. The growth suspension (spore or mycelia) were blended in blender under sterilized conditions. The number of spores or mycelial fragments in the stock suspension was counted with a haemocytometer slide and adjusted to 106 cfu or mycelial fragments / ml . One ml of growth suspensions was added to Screw-cap glass vials, 20 cm long and 20 mm in diameter, containing 20.0 ml sterilized water placed in water path at 25, 50, 52, 54, 56, and 58 oC, for different exposures times i. e. 1, 10, 20, and 30 minutes. One ml of treated suspension was transferred into Petri plates (9 cm diameter) and sterilized PDA medium before its solidification disbanded in Petri- plates which containing treated growth suspensions . Plates were incubated at 25°C for 5 days. Plates showing growth or non- growth were recorded. Effect of hot-water treatment on resting stage viability of tomato soil borne fungi:
Different hot water temperatures i.e. 25, 54, 56, 58, 60 and, 62 oC, for exposures time i. e, 1, 5, 10, 15,
20, 25 and 30 minutes were tested to study their effect on the resting stage germination of F. solani, F. oxysporum f.sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici (FORL), R. solani and S. rolfsii under laboratory conditions. Effect on sclerotia of S. rolfsii:
Sclerotia of S. rolfsii were harvested and surface disinfected with Ethanol alcohol (70 %) for 3 sec, then
washed with sterilized water several times. Sclerotia were transferred to glass vials in digital water path at different temperatures and exposure times as mentioned before. Treated sclerotia were dried using sterilized filter paper and transferred to Petri-plates containing PDA medium. Determination of sclerotia germination was carried out according to the method described by Edmunds and Gleason, (2003).Ten sclerotia were distributed evenly on the surface of each Petri plate. The plates were incubated at 25C for 5 days. Sclerotia were considered to have germinated if the white, mycelium characteristic of S. rolfsii was presented after 5 days. Percentage of sclerotia germination was recorded. Effect on sclerotia of R. solani:
Sclerotia of R. solani were harvest and surface disinfected with Ethanol alcohol (70 %) for 3 sec, then
washed with sterilized water several times. Sclerotia were transferred to glass vials in digital water path at different temperatures and exposure times as mentioned before. Treated and un treated sclerotia were dried on sterilized filter paper. Determination of sclerotia germination was carried out according to the method described by Demirci et al., (2009). The sclerotia were placed on the Petri plates, and incubated at 20 oC in a sterile humidity chamber (100% rh). After 30 days, the viability of R. solani sclerotia was estimated by placing them on PDA medium for 5 days at 25 oC. Percentage of sclerotia germination was recorded. Effect on chlamydospores of Fusarium spp:
Chlamydospores suspension was prepared by culturing F, salami, F. oxysporum f.sp. lycopersici ( FOL)andF. oxysporum f.sp. radicis lycopersici( FORL) on Petri-plates containing water agar medium for 20 days at
Middle East j. Appl. Sci., 3(3): 105-112, 2013
25°C. Colony forming units (cfu) containing Chlamydospores were released in sterilized water using a needle and 1 ml of suspension was transferred to Screw-cap glass vials, 20 cm long and 20 mm in diameter, containing 20.0 ml sterilized water placed in water path at different temperatures and exposure times as mentioned before. One ml of treated chlamydospores suspension was transferred to test tube containing sterilized broth PD medium. Test tubes were incubated at 25°C for 24 h. One ml of treated colony forming units ( cfu) containing chlamydospores was examined microscopy and percent of chlamydospores germination was calculated. Effect of sublethal temperatures on linear growth of tomato soilborne fungi:
Agar disks with mycelia of F. solani, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici (FORL), R. solani and S. rolfsii were exposed to sublethal temperatures i.e. 56.0, 54.0, 54.0, 52 and 54.0 respectively, for 10 minutes (as mentioned before). Optimum temperatures (25.0 - 27 oC) for all tested fungi served as control. Petri plates (9 cm – diameter) containing PDA medium were individually inoculated at the center with treated growth agar disks. Five plates were used as replicates for each particular treatment. Inoculated plates were incubated at 25 ± 2 °C. The average linear growth of fungi was calculated every two days. Effect of sublethal temperatures on resting stage production of tomato soilborne fungi:
Agar disks with mycelia of F. solani, F. oxysporum f.sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici (FORL), R. solani and S. rolfsii were exposed to sublethal temperatures i.e. 56.0, 54.0, 54.0, 52 and 54.0 respectively for 10 minute (as mentioned before). Optimum temperatures (25.0 - 27 oC) for all tested fungi served as control. Petri plates (9 cm – diameter) containing PDA medium were individually inoculated at the center with treated growth agar disks. Five plates were used as replicates for each particular treatment. Inoculated plates were incubated at 25 ± 2 °C for 30 days . Production of chlamydospores or sclerotia / cm2 was estimated. Pot experiments: Effect of sublethal temperature of hot water treatments on pathogenic ability of tomato soil-borne fungi under greenhouse conditions:
Agar disks with mycelia of F. salami, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici (FORL), R. solani and S. rolfsii were exposed to sublethal temperatures i.e. 56.0, 54.0, 54.0, 52 and 54.0 respectively for 10 minute (as mentioned before). Optimum temperatures (25.0 oC) for all tested fungi served as control. Growth of treated fungi were maintained on PDA medium Inoculum preparation, and soil infestation
Inocula of R. solani, F. solani, S. rolfsii and P. ultimum were prepared by culturing each fungus on 50.0
ml potato dextrose broth (PDB) medium in 250 ml Erlenmeyer flasks for 15 days at 25° - 27 oC. and fungal inocula were prepared as follows:
Inoculum of F. solani was prepared from the growing upper solid layers which washed and blended in
sterilized water .Colonies forming units (cfu) were adjusted to 10 6 cfu / ml using haemocytometers slide. Soil infestation was carried out at rate of 50 ml (10 6 cfu / ml ) / kg soil (Elad and Baker, 1985).
Inoculumof S. rolfsii and R. solani was prepared from the growing upper solid layers which washed and
air-dried with sterilized filter paper layers. The air-dry mycelium was blended in distilled water to obtain inocula pieces of 1-2 mm in diameter. Soil infestation was carried out at rate of 2.0 g dry mycelium / kg soil, (Al-Mahareeq, 2005).
Inoculum of P. ultimum was prepared from the growing upper solid layers which washed and blended in
distilled water. Propagules were adjusted to 106 / ml using haemocytometers slide. Soil infestation was carried out at rate of 50 ml (106 Propagules/ ml ) / kg soil (Lu et al., 2004). Soil infestation:
Sandy -loamy soil was autoclaved at 120°C for 1 h on three successive days. Plastic pots (30 cm diameter,
5.0 kg soil) containing sterilized sandy-loamy soil were artificially infested individual with the inoculm of each fungus as mentioned before. Eight pots were used as replicates for each treatment as well as check treatment (un- infested soil). Disinfected cucumber seeds, c.v. Beit Alpha, were sown at the rate of 8 seeds / pot. Root rot disease was recorded as percentages of diseased plants after 20 and 40 days of sowing date. Statistical analysis: Middle East j. Appl. Sci., 3(3): 105-112, 2013
Tukey test for multiple comparison among means was utilized (Neler, et al.,1985).
Results: Effect on mycelia agar disks and growth suspension:
Viability of agar disks with mycelia and growth suspension of R. solani, F. solani, F. oxysporum f. sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici( FORL) ,and S. rolfsii were tested against different temperatures i.e. 25, 50, 52, 54, 56, and 58 oC and exposure times i. e, 1, 10, 20, and 30 minutes in digital water path. Results in Table (1 and 2) indicate that growth (spores or mycelial ) suspension more sensitive than disks of agar to high temperatures and exposure times . When exposures times increased the lethal temperatures of hot water decreased for all tested fungi. The lethal temperatures to R. solani , F. solani and S. rolfsii were 54.0 , 58.0 or 56 oC and 52.0 , 56.0 or 54.0 oC when were exposed to temperatures for one minutes as agar disks or growth suspension respectively .Meanwhile, the lethal temperatures to F. oxysporum f. sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici( FORL)were 56 oC and 54 oC when were exposed to temperatures for one minutes as agar disks or growth suspension respectively Table 1: Viability of mycelia agar disks of tomato soil borne fungi as affected with hot water temperatures and exposure times.
ــــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ
ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ
1- (+) = Indicate growth (-) = Indicate no growth Table 2: Viability of growth suspension of tomato soil borne fungi as affected with hot water temperatures and exposure times.
ـ ــ ــــ ـ ــ ـ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ
ــ ـ ــ ـ ــ ـ ــ ـ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ ـ ــ
1- (+) = Indicate growth (-) = Indicate no growth
Viability of resting stage of tomato soil borne fungi as affected with hot water temperatures and exposure times:
Different hot water temperatures i.e. 25, 54, 56, 58, 60 and 62 oC, for exposures time i. e, 1, 10, 20 and 30
minutes were tested to study their effect against resting stage germination of cucumber root rot fungi under laboratory conditions. Results in Table (3) indicate that when exposure times increased the lethal temperatures of hot water decreased for Chlamydospores and Sclerotia. Chlamydospores are more resistant to high temperatures as they were killed at 62 and 60 oC for F. solani and FOL or FORL respectively. While Sclerotia were killed at 58.0 oC for R. solani and S. rolfsii when exposed to hot water for one minutes. Effect of sublethal temperatures on tomato soil borne fungi:
Effect of sublethal temperatures on linear growth and resting stage germination of R. solani, F. solani, F. oxysporum f. sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici( FORL), and S. rolfsii were tested. Effect on linear growth of tomato soil borne fungi:
Agar disks with mycelia of F. solani, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici( FORL), R. solani and S. rolfsii were exposed to sublethal temperatures i.e. 56.0, 54.0, 54.0, 52 and 54.0 respectively, for 10 minutes to study their effect on linear growth of tomato root fungi. Results in Table
Middle East j. Appl. Sci., 3(3): 105-112, 2013
(4) indicate that sublethal temperatures significantly reduced the linear growth of all tested fungi. They reduced the linear growth of F. solani, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici (FORL) more than 50 % as compared with optimum temperatures.
Table 3: Viability of resting stage of tomato soil borne fungi as affected with hot water temperatures and
1- (+) = Indicate growth (-) = Indicate no growth Table 4: Linear growth ( mm) of tomato soil borne fungi exposed to sublethal temperatures.
Figures with the same letter are not significantly different , to compare between optimum and sublethal temperatures of each fungus (P = 0.05) Effect on resting stage production:
The effect of exposure resting stage of F. solani, F. oxysporum f.sp. lycopersici ( FOL), F. oxysporum f.sp. radicis lycopersici( FORL), R. solani and S. rolfsii to sublethal temperatures was shown in Table (5) Results show that sublethal temperatures significantly reduced all resting stage production. Exposure of resting stage ofF. solani, F. oxysporum f.sp. lycopersici (FOL), F. oxysporum f.sp. radicis lycopersici( FORL) growth to sublethal temperature caused reduction in chlamydospores production by 61.0, 59.7 and 60.4 % respectively. Meanwhile exposure of resting stage of S. rolfsii and R. solani resulted in reducing Scleritia production by 57.1 and 50.0 % respectively.
Table 5: Average number of resting stage production of tomato soil borne fungi exposed to sublethal temperatures. F. oxysporum f. sp.radicis lycopersici
Figures with the same letter are not significantly different , to compare between optimum and sublethal temperatures ( P = 0.05 ) Effect of sublethal temperature on pathogenic ability of Tomato soil borne fungi under greenhouse conditions: Results in Table (6) indicate that sublethal temperatures significantly reduced the root rot and wilt diseases
for all tested fungi if compared with nrmal temperature (25 oC). It caused reduction in disease incidence more than 84.4 % for all tested fungi.
Middle East j. Appl. Sci., 3(3): 105-112, 2013Table 6: Pathogenic ability of cucumber root rot fungi as affected with sublethal temperatures of hot water treatments. F. oxysporum f. sp.radicis lycopersici
1- Figures with the same letter are not significantly different , to compare between optimum(* *) and sublethal( * ) temperatures of each fungus (P = 0.05) Discussion:
Tomato soil borne pathogenic fungi consider the most damaging soil-borne diseases of tomato and
becoming more common in greenhouse tomato production. Both diseases caused a significant threat to tomato transplant production and to both tomato field and greenhouse fruit production, wherever it accord (McGovern et al., 1998). Fusarium grown and root rot of tomato caused by Forl killed about 70-83% of tomato young plants causing rot and basal stem decay and eventually death (Kuckareck et al., 2000).
Soil solarization during summer months increases soil temperatures to lethal levels for many soil-borne
plant pathogens, nematodes and weeds, (Primo and Cartia, 2001; Abd-El-Kareem et al., 2004; Culman, et al, 2006 and Farag and Fotouh, 2010). The inability of organisms to tolerate high temperatures is related to an upper limit in the degree of fluidity of membranes, beyond which breakdown of membrane function may be associated with membrane instability (Sundarum, 1986). Additional causes for the thermal decline of microorganisms at high temperatures involve the sustained inactivation of respiratory enzymes (Brock, 1978 and Sundarum, 1986). These are direct effects of high soil temperatures and account for a major share of the reduction in populations of soil- borne micro-organisms and weed seeds. On the other hand, some effects of soil solarization or hot water are indirect. For example, cells of plant pathogens weakened by heat stress are more vulnerable by several orders of magnitude to soil fumigants, to antagonistic micro-organisms which are more able to tolerate high soil temperatures, and to changes in the gas environment which may develop during soil solarization. During heat treatments of soil, changes occur in the structure of soil, in soluble mineral substances available for plant and microbial growth, and in the populations of soil-borne micro-organisms (Chen, and Katan, 1980, Stapleton, and DeVay, 1984 and Stapleton, et al., 1985). These changes affect the inoculum density of plant pathogens, and also their aggressiveness and survival. Changes in the populations of other soil - borne micro-organisms occur during and after solarization which may influence the disease suppressive of soil and also the increased plant growth response associated with heat treatments of soil (Katan, 1987, Stapleton, and DeVay. 1984 and Stapleton, et al., 1985).
In the present study, under laboratory conditions, results indicated that the lethal temperatures to R. solani , F. solani and S. rolfsii were 54.0, 58.0 or 56 oC and 52.0, 56.0 or 54.0 oC when were exposed to temperatures for one minutes as agar disks or growth suspension respectively. Meanwhile, the lethal temperatures to F. oxysporum f. sp. lycopersici ( FOL)and F. oxysporum f.sp. radicis lycopersici (FORL) were 56 oC and 54 oC when were exposed to temperatures for one minutes as agar disks or growth suspension respectively. Chlamydospores are more resistant to high temperatures as they were killed at 62 and 60 oC for F. solani and FOL or FORL respectively. While Sclerotia were killed at 58.0 oC for R. solani and S. rolfsii when exposed to hot water for one minutes. Sublethal temperatures significantly reduced the linear growth and reduced all resting stage production of all tested fungi.
Sublethal temperatures also may cause delays in germination of propagules and reduced virulence in host
plants that vary with temperature and the duration of exposure. In the present study results indicated that sublethal temperatures significantly reduced linear growth and resting stage production for all tested fungi . In this respect Pullman et al., (1981) found that the effects of sublethal temperatures were pronounced when the fungi were exposed to temperatures of 37° to 39°C. Propagule was exposed to sublethal heating, the longer time was required for germination. Moreover, they suggested that the heat damage accumulates gradually to a point beyond which the propagule cannot recover. During sublethal heating, all living cells produce heat shock proteins (Freeman, et al., 1989, Lindquist, 1986 and Plesofsky-vig, and Brambl, 1985). Heat shock proteins are associated with the acquisition of thermo tolerance or thermos/ability; however, fungi have a transient heat shock response that is short live, even if they are maintained at high temperature (Plesofsky-vig, and Brambl. 1985). The overall effect of heat shock proteins on the survival of fungi during soil solarization is unknown. Other effects of sublethal heating are well documented, especially in the case of Sclerotium rolfsii where the
Middle East j. Appl. Sci., 3(3): 105-112, 2013
rind of sclerotia becomes cracked resulting in increased leakage of various substances (Lifshitz, et al., 1983). Weakened sclerotia are intensely colonized by Trichoderma harzianum and other micro-organisms (Greenberger et al., 1984 and Lifshitz, et al., 1983). Another example where soil solarization may affect the germination ability and aggressiveness of fungal propagules concerns Rosellinia necratrix. Post plant solarization of an apple orchard for the control of this pathogen provided evidence that the fungal propagules became highly vulnerable to colonization by Trichoderma species (Sztejnberg, et al., 1987). Acknowledgment
This work was supported financially by Ministry of Scientific Research , Egypt, Grant No. 10/4/10.
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LIFE SCIENCES PAPER MEMORANDUM 1 Tissues, cells & molecular studies and Life Systems SECTION A: QUESTION 1 1.1.1 C 1.1.2 D √√ 1.1.3 A √√ 1.1.4 A √√ 1.1.5 C √√ 1.2.4 bivalent or homologous chromosomes √ 1.2.5 amniocentesis 1.3.3 B √ 1.3.4 A √ 1.3.5 D √ 1.4.1 C,E, D, B, F, A √ mark each 1.4.2 crossing over increases variation √
Weekly e Briefing: 22 February 2013 Welcome to the Commissioner’s weekly horizon scanning brief: 1. Legislation (Legislation, Home Office, APCC, press comments, reports and campaigns relating to strategy, policy and programmes) 2. Policing and crime key developments (relevant crime and criminal justice information and partners’ policy/reports/campaigns) 3. Reports (c