Abstract:
The present invention addresses the need to effectively produce high volumes of desiccation tolerant spores of fungal species such as Paecilomyces fumosoroseus. The present invention accomplishes this by providing a liquid culture media optimally enriched in nitrogen and carbon.

Description:
RELATED APPLICATION 
     This application is a continuation of application Ser. No. 08/623,915, filed on Mar. 28, 1996, now abandoned which is a continuation-in-part of U.S. patent application Ser. No. 08/499,481, filed Jul. 7, 1995, now abandoned. 
    
    
     FIELD OF THE INVENTION 
     The present invention pertains generally to methods and compositions related to the control of soft-bodied insect pests. The invention especially concerns methods and compositions for producing and drying desiccation-tolerant Paecilomyces fumosoroseus spores for controlling Bemisia tabaci (sweetpotato whitefly) and other soft-bodied insect pests. 
     BACKGROUND OF THE INVENTION 
     Myriad approaches have been pursued to control pests. Many of these approaches are directed to the control of pests that attack plants, most notably commercially valuable plants. Although much current agricultural research has pest control as its objective, pest destruction of plants and plant products is still a major problem. 
     Chemical pesticides in particular have been used extensively to control pests for many years. An awareness of recent problems associated with the use of chemical pesticides such as adverse effects on man and the environment has led to a focus on biological control alternatives to chemical pesticides. For instance, certain fungi have been identified to be pathogenic to different pests. Importantly, many fungi, unlike pathogenic bacteria, viruses and protozoa need not necessarily be ingested by the target insect to initiate disease, but instead usually invade through their host&#39;s cuticle. 
     Sweetpotato whitefly is a particularly serious insect pest worldwide. In Texas and California alone, agronomic losses exceed $250 million annually. The insect rapidly develops resistance to chemical pesticides and is not adequately controlled with current pest management practices. 
     Various strains of the fungus Paecilomyces fumosoroseus have been proposed as a possible biological control agent for sweetpotato whitefly. A significant constraint to the development of this fungus and other like fungi as biocontrol agents, however, is the availability of low-cost methods for producing infective propagules. Solid-substrate methods of producing spores from such fungi as Paecilomyces fumosoroseus have proven too costly for commercial consideration. Hence, liquid culture methods for producing spores are preferred. 
     Eyal et al. has described in U.S. Pat. No. 5,360,607 a submerged culture technique for growing the mycelium of Paecilomyces fumosoroseus. The grown mycelial biomass is harvested and then formed into dry prill which can be used directly on plants and soil or the prill can be used as a carrier for sporulation of conidia spores. However, to be an effective insecticidal agent, mycelia containing prill must be wetted, the fungus must grow and sporulate, and insects must contact the newly formed spores. It would be more advantageous to develop a method of producing a high volume of insecticidal spores (versus mycelium) which could be directly applied to insects and actively instigate insect kill without the need for sporulation and contact by the target insect. 
     Previous attempts to produce Paecilomyces fumosoroseus spores directly using liquid culture fermentation methods have yielded unstable spores which are desiccation intolerant and hence readily perish during drying. Clearly, there is a need to develop a method to rapidly produce high volumes of spores which are desiccation tolerant and have high survival rates after drying and storage. In particular, it would be useful to produce desiccation tolerant spores of Paecilomyces fumosoroseus. 
     SUMMARY OF THE INVENTION 
     The present invention addresses the need to effectively produce high volumes of desiccation tolerant spores of fungal species such as Paecilomyces fumosoroseus. Specifically, the invention provides a liquid culture medium which allows for the rapid production of a high volume of desiccation resistant fungal spores and a method of producing the same. 
     In a first general embodiment, the invention provides a liquid culture medium for producing a high concentration of desiccation resistant fungal spores, whereby the medium comprises a nitrogen source at a concentration between 8.1 grams/liter and less than 50 grams/liter. The nitrogen source is preferably selected from the group consisting of hydrolyzed casein, yeast extract, hydrolyzed soy protein, hydrolyzed cottonseed protein, hydrolyzed corn gluten protein, and other nitrogen sources. 
     In a preferred embodiment the nitrogen source is present at a concentration greater than 12.5 grams/liter and optimally, at a concentration between 13.2 grams/liter and 30 grams/liter. In an especially preferred embodiment, the liquid culture medium further comprises a carbon source greater than 20 grams/liter and most optimally, greater than or equal to 80 grams/liter. In a most preferred embodiment the liquid culture medium comprises a nitrogen source at a concentration between 13.2 grams/liter and 30 grams/liter and a carbon source greater than or equal to 80 grams/liter. 
     In a second general embodiment the invention provides a liquid culture medium for producing a high concentration of desiccation resistant Paecilomyces fumosoroseus spores whereby the medium comprises a nitrogen source present at a concentration between 8.1 grams/liter and less than 50 grams/liter. 
     The nitrogen source is preferably selected from the group consisting of hydrolyzed casein, yeast extract, hydrolyzed soy protein, hydrolyzed cottonseed protein, and hydrolyzed corn gluten protein. 
     In a preferred embodiment the nitrogen source is present at a concentration greater than 12.5 grams/liter and optimally, at a concentration between 13.2 grams/liter and 30 grams/liter. In an especially preferred embodiment, the liquid culture medium further comprises a carbon source greater than 20 grams/liter and most optimally, greater than or equal to 80 grams/liter. In a most preferred embodiment the liquid culture medium comprises a nitrogen source greater than 13.2 grams/liter and a carbon source greater than or equal to 80 grams/liter. 
     The present invention further contemplates a method of producing a high concentration of desiccation tolerant fungal spores, comprising the steps of inoculating liquid culture medium comprising a nitrogen source with fungal propagules, whereby the nitrogen source is between 8:1 and less than 50 grams/liter; incubating the propagules for a sufficient time to allow for maximum sporulation; collecting the resulting spores; and drying the spores. 
     The nitrogen source is preferably selected from the group consisting of hydrolyzed casein, yeast extract, hydrolyzed soy protein, hydrolyzed cottonseed protein, and hydrolyzed corn gluten protein. 
     In a preferred embodiment the nitrogen source is present at a concentration greater than 12.5 grams/liter and optimally, at a concentration between 13.2 grams/liter and 30 grams/liter. In an especially preferred embodiment, the liquid culture medium further comprises a carbon source greater than 20 grams/liter and most optimally, greater than or equal to 80 grams/liter. In a most preferred embodiment the liquid culture medium comprises a nitrogen source greater than 13.2 grams/liter and a carbon source greater than or equal to 80 grams/liter. 
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS 
     FIG. 1 depicts a time plot of blastospore production in medium containing 80 grams glucose/liter and 13.2 grams hydrolyzed casein/liter. 
     FIG. 2A depicts glucose utilization plotted against time for Paecilomyces fumosoroseus in medium containing 80 grams glucose/liter and 13.2 grams hydrolyzed casein/liter. 
     FIG. 2B depicts amino acid utilization plotted against time for Paecilomyces fumosoroseus in medium containing 80 grams glucose/liter and 13.2 grams hydrolyzed casein liter. 
     FIG. 3 depicts the percentage viability of spores air-dried at various relative humidities and stored at 4° C. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     Fungi have recently been recognized as a valuable potential source for natural antiinsectons. Specifically, spores of certain fungi have been shown to contain metabolites that exert adverse physiological effects on insects. While spores from certain fungi hold great promise as biocontrol agents, a particular problem with such natural agents is the ability to rapidly produce a high volume of stable spores at low cost and which can be dried and stored without loss of activity. 
     A particularly serious insect pest is Bemisia tabaci. Bemisia tabaci Gennadius (Sweetpotato whitefly, cotton whitefly) has been reported to attack over 600 plants in warm climates worldwide (Smith, 1993). The ability of this phloem-feeding insect to reproduce rapidly can lead to heavy infestations which are capable of killing the host plant. Resistance to chemical insecticides and a lack of natural enemies has made the sweetpotato whitefly a serious pest in the Southern United States (Lacey, Kirk, and Hennessey, 1993). Predacious insects and entomopathogenic fungi are being evaluated as potential biological control agents for this pest. In general, the heavy use of insecticides in cropping systems where whiteflies are problematic has precluded the use of predacious insects. Fungi, which penetrate the cuticle of the insect, such as Paecilomyces fumosoroseus, appear to offer the best opportunity for biological control. 
     Many strains of Paecilomyces fumosoroseus and Beauveria bassiana have been isolated that are aggressive pathogens of numerous soft-bodied insects including B. tabaci (Lacey, Kirk, and Hennessey, 1993; Puterka, Humber, and Poprawski, 1994). Table 1 lists various Paecilomyces fumosoroseus strains and their countries of origin. 
     
                                           TABLE 1__________________________________________________________________________Yield and Desiccation Tolerance of Liquid-Culture-Produced  Spores of Various Paecllomyces Fumosoroseus Strains.sup.1  P. fumosoroseus STRAINPaecilomyces  Fumosoroseus Strain    VIABLE FREEZE-  ARSEF OTHER LOCATION OF YIELD FREEZE-DRYING.sup.2 DRIED SPORES.sup.2                                DESIGNATION COLLECTION (spores/ml)                               (% SURVIVAL) (spores/ml)__________________________________________________________________________4490    Ma8   INDIA: PADAPPAI                1.09E + 09                      78       8.55E + 08  4491 Ma17 INDIA: PADAPPAI 6.78E + 08 88 6.03E + 08  4492 Ma18 INDIA: PADAPPAI 4.43E + 08 88 3.90E + 08  4493 Ma19 INDIA: PADAPPAI 5.35E + 08 89 4.83E + 08  4494 Ma20 INDIA: PADAPPAI 6.18E + 08 89 5.50E + 08  4495 Ma21 INDIA: PADAPPAI 4.25E + 08 85 3.60E + 08  4496 Ma22 INDIA: PADAPPAI 6.48E + 08 88 5.78E + 08  4497 Ma27 INDIA: PADAPPAI 7.20E + 08 73 4.60E + 08   Pfr92111 PAKISTAN: MULTAN 8.65E + 08 76 6.38E + 08   Pfr92116 PAKISTAN: MULTAN 4.06E + 08 87 3.57E + 08  3377 Pfr92117 PAKISTAN: MULTAN 7.00E + 08 86 6.00E + 08  3878 Pfr92118 PAKISTAN: MULTAN 3.75E + 08 90 2.76E + 08   Pfr92119 PAKISTAN: MULTAN 5.95E + 08 78 4.43E + 08  3870 Pfr92133 NEPAL: KATMANDU 5.20E + 08 92 4.78E + 08    VALLEY   Pfr92134 NEPAL: KATMANDU 4.48E + 08 82 3.75E + 08    VALLEY  3871 Pfr92135 NEPAL: KATMANDU 4.80E + 08 89 4.28E + 08    VALLEY   Pfr92136 NEPAL: KATMANDU 4.76E + 08 92 4.36E + 08    VALLEY   Pfr92138 NEPAL: KATMANDU 6.23E + 08 86 4.90E + 08    VALLEY  4480 Pfr3660 CALIFORNIA: 5.08E + 08 91 4.78E + 08    EL CENTRO  4481 Pfr3663 CALIFORNIA: 3.40E + 08 95 3.28E + 08    CALEXICO  4489 Pfr3698 CALIFORNIA: 4.65E + 08 96 4.48E + 08    CALEXICO   Pfr3572 TEXAS: McALLEN 6.05E + 08 92 5.65E + 08   Pfr3594 TEXAS: McALLEN 3.93E + 08 82 3.40E + 08  FPLSD.sup.3 (P &gt; 0.05) =  3.53E + 08 NSD.sup.4 NSD__________________________________________________________________________ .sup.1 SPORES COLLECTED FROM 4DAY OLD CULTURES. .sup.2 SPORE VIABILITY DETERMINED BY 6 HOUR GERMINATION ASSAY IN POTATO DEXTROSE BROTH. .sup.3 FISHER&#39;S PROTECTED LEAST SIGNIFICANT DIFFERENCE. .sup.4 NOT SIGNIFICANTLY DIFFERENT. 
    
     The feasibility of using P. fumosoroseus as biocontrol agents against sweetpotato whitefly is dependent on numerous biological constraints, including the ability to produce high concentrations of stable propagules at a reasonable cost (Jaronski, 1985; Latge et al., 1985). On solid substrates, Paecilomyces fumosoroseus and Beauveria bassiana strains produce abundant aerial conidia which are amenable to storage as dry preparations. In submerged culture, Paecilomyces fumosoroseus, Paecilomyces farinosus, and Beauveria bassiana are reported to produce high concentrations of spores (Bidochka, Pfeifer, and Khachatourians, 1987). Spores produced in liquid culture by various entomopathogenic fungi are typically larger than aerial conidia, are not amenable to simple drying techniques, and tend to perish more rapidly during storage (Inch et al., 1986; Inch and Trinci, 1987; Lane, Trinci, and Gillespie, 1991; Hegedus et al., 1992). 
     The present invention has focused on developing liquid culture techniques for producing desiccation tolerant spores such as spores from Paecilomyces fumosoroseus as well as other species. Various liquid culture medium were evaluated for producing Paecilomyces fumosoroseus spores based on spore yield and stability as a dry preparation. A liquid culture medium was identified which supported the rapid production of high concentrations of desiccation tolerant Paecilomyces fumosoroseus spores which were capable of infecting and killing the sweetpotato whitefly, B. tabaci and other soft bodied insects including Russian wheat aphid Agropyron elongatum and greenhouse whitefly (Trialeurodes vaporariorum). 
     Optimal Composition of Liquid Culture Medium for Spore Production 
     The impact of nutrition on submerged culture production of desiccation tolerant Paecilomyces fumosoroseus spores was evaluated by growing the fungus in media with differing carbon concentrations and carbon-to-nitrogen (CN) ratios. Spores were produced by inoculating liquid culture medium with fungal propagules; incubating the propagules, and collecting and drying the spores. Propagules are any living cells from a fungus that will propagate such as spores, mycelium or other fungal biomass. 
     
                                           TABLE 2__________________________________________________________________________Evaluation of Liquid Culture Spore Production and Desiccation  Tolerance by Paecllomyces Fumosoroseus ARSEF 4491 Using VariousMedia.sup.1       AMINO       CARBON   CASAMINO ACID TO-  GLUCOSE ACIDS MIXIURE.sup.4 [CARBON] NITROGEN PRODUCTION.sup.2 AIR-DRYIN                                 G.sup.3  (g/L) (g/L) (g/L) (g/L) RATIO (106 spores/ml) (% SURVIVAL)__________________________________________________________________________80.0  13.2  --    39    36:1  580.sup.a#                                 79.sup.a  3.6 1.7 -- 4 30:1 46.sup.b,c 6.sup.b,c  7.8 5.0 -- 4 10:1 94.sup.b,c 30.sup.b  9.2 0.6 -- 4 80:1 15.sup.c    3.sup.c  15.6 -- 3.2 8 15:1 130.sup.b   32.sup.b__________________________________________________________________________ .sup.1 ALL MEDIA CONTAINED THE BASAL COMPONENTS LISTED IN THE MATERIALS AND METHODS. .sup.2 THREEDAY-OLD CULTURES. .sup.3 AIRDRYING OVERNIGHT WITH AIR (RH 20-30%). WHOLE CULTURE MIXED WITH 5% (w/v) DIATOMACEOUS EARTH. .sup.4 SYNTHETIC AMINO ACID MIXTURE. MIXC, JACKSON &amp; SLININGER. 1993. J. IND. MICROBIOL. 12:417-422. .sup.# VALUES IN COLUMNS FOLLOWED BY DIFFERENT LETTERS ARE SIGNIFICANTLY DIFFERENT USING FISHER&#39;S PROTECTED LSD. 
    
     As shown in Table 2, significantly higher concentrations of Paecilomyces fumosoroseus spores were produced in media which contained a high concentration of carbon and nitrogen. Under the conditions of this study, optimal production occurred at a carbon level of 80 grams glucose/liter and a nitrogen level of 13.2 grams Casamino acids/liter. Casamino acids are amino acids derived by hydrolyzing the protein casein. Media having 80 grams glucose/liter and 13.2 grams Casamino acids/liter will hereinafter be referred to as MS media. Such media, also enhanced spore tolerance to desiccation. 
     In addition to glucose, most carbohydrates tested in medium containing 13.2 grams hydrolyzed casein/liter allowed for excellent spore germination and desiccation resistance after freeze drying. Table 3 shows a comparison of Paecilomyces fumosoroseus ARSEF 4491 spore yield and desiccation tolerance when propagules were grown on various carbon sources. 
     
                       TABLE 3______________________________________Comparison of Paecllomyces Fumosoroseus ARSEF 4491 spore yield  and Desiccation Tolerance When Grown on Other Carbon Sources.sup.1                  AFTER                   SPORE YIELD FREEZE-DRYING  (spores/ml) spore germination (%)______________________________________GLUCOSE     6.7E + 08  82.5  FRUCTOSE 3.7E + 08 92.0  SUCROSE 5.0E + 08 72.5  GALACTOSE 2.9E + 08 86.5  GLYCEROL 7.4E + 08 92.0  CITRATE 1.9E + 08 71.0  ACETATE 0.0E + 00 0.0______________________________________ .sup.1 The standard production medium and conditions were used. 80 g Glucose/L is replaced by 80 g/L of the various carbon sources. 
    
     Likewise, suitable nitrogen sources are not limited to hydrolyzed casein. Table 4 shows that numerous nitrogen sources support the liquid culture production of high concentrations of spores with improved desiccation tolerance after drying. Benefical sources of nitrogen include yeast extract, hydrolyzed casein, soy protein, cottonseed protein and corn gluten protein. 
     
                       TABLE 4______________________________________Effect of Nitrogen Source on P. fumosoroseus  Blastospore Yield and Desiccation Tolerance.sup.#           Blastospore                      After Freeze-                                Viable  Nitrogen Yield drying spores/ml  Source (spores/ml) (% germination)* (after drying)______________________________________Yeast Extract       9.9E + 08  79          7.8E + 08  Enhancetone 1.2E + 09 43 5.3E + 08  Casamino Acids 6.0E + 08 82 4.8E + 08  Papaic Digest of Soy 1.1E + 09 38 4.6E + 08  Cottonseed 7.7E + 08 50 4.1E + 08  Hydrolysate  Corn Gluten 5.6E + 08 58 3.4E + 08  Hydrolysate  Corn Steep Liquor 4.0E + 08 44 2.3E + 08  Digest of Milk &amp; 4.4E + 08 50 1.9E + 08  Meat Protein  Distiller&#39;s Dried 4.5E + 08 56 1.9E + 08  Grains &amp; Solubles  Digest of Rice Flour 1.0E + 08 15 1.8E + 08  LSD P = 0.05 2.5E + 08 31 2.9E + 08  LSD P = .01 3.4E + 08 42 3.9E + 08______________________________________ .sup.# Basal salts liquid medium with 80 g glucose/L and 13.2 g nitrogen source/L. Incubated 28° C. and 300 rpm. *6hour germination assay  Potato Dextrose Broth, 28° C., 300 rpm. 
    
     The experiments that produced the data shown in Tables 3 and 4 were run using the standard production medium and conditions detailed in Examples 1 and 2 of this application. 
     When cultures were grown in media supplemented with glucose and Casamino acids in which the carbon concentration was held constant (4 g carbon/liter) and the CN ratio varied, lower concentrations of desiccation sensitive spores were produced. In medium with 4 g carbon/liter, spore concentrations were not significantly different regardless of the CN ratio of the medium and desiccation tolerance was only slightly better in spores produced in medium with a CN ratio of 10:1 when compared to spores produced in medium with a CN ratio of 80:1 (Table 2). 
     It is suspected that nitrogen depletion may limit sporulation since spore concentrations did not significantly increase after amino acids were utilized (FIG. 2). Furthermore, when glucose levels were held constant at 80 grams/liter, sporulation increased with increasing Casamino acid concentration up to 25 grams/liter as shown in Table 5. Upon further experimentation, premium sporulation was achieved with a Casamino acid concentration of 40 grams/liter and up to 50 grams/liter as shown in Table 5A. Specifically, 13.2 to 30 grams Casamino acids/liter appeared to be necessary for maximum spore yield while greater than or equal to 6.8 grams Casamino acids/liter and less than 50 grams/liter casamino acids appeared to be necessary for maximal viability after drying. 
     
                       TABLE 5______________________________________Effect of Casamino Acid Concentration on Sporulation and  Desiccation Tolerance of Paecilomyces fumosoroseus 4491 Blastospores.sup.1  Casamino               Viability After                               Viable Spores  Acids Blastospore Yield.sup.2 Drying.sup.3 (% After Drying  (g/L) (spores/ml) spore germination) (spores/ml)______________________________________25.0    4.0E + 07    59           2.4E + 07  20.0 7.5E + 08 85 6.3E + 08  15.0 4.3E + 08 76 3.3E + 08  13.2 4.6E + 08 83 3.7E + 08  11.4 2.7E + 08 79 2.2E + 08  9.6 2.4E + 08 85 2.0E + 08  6.8 1.5E + 08 78 1.2E + 08  5.0 8.5E + 07 58 4.8E + 07  3.2 6.7E + 07 49 3.0E + 07  1.4 5.3E + 07 10 4.8E + 06______________________________________ .sup.1 Cultures grown in basal salts liquid medium with vitamins and 80 g glucose/L. .sup.2 4 dayold cultures. .sup.3 Spores mixed with diatomaceous earth, dewatered, and airdried at 25° C. and a relative humidity of 65%. Viability determined with 6hour germination assay. 
    
     
                       TABLE 5A______________________________________Effect of Casamino Acid Concentration on Sporulation and  Desiccation Tolerance of Paecilomyces fumosoroseus 4491 Blastospores.sup.1  Casamino               Viability After                               Viable Spores  Acids Blastospore Yield.sup.2 Drying.sup.3 (% After Drying  (g/L) (spores/mL) spore germination) (spores/mL)______________________________________50      3.0E + 07    ND.sup.4     ND  40 6.4E + 08 56 3.9E + 08  30 7.3E + 08 71 5.2E + 08  25.0 8.9E + 08 68 6.1E + 08  20.0 7.2E + 08 80 5.8E + 08  15.0 5.8E + 08 68 3.9E + 08  13.2 5.8E + 08 79 4.6E + 08  10 4.4E + 08 31 1.3E + 08  5.0 3.4E + 08  6 2.0E + 07FPLSD.sup.5   2.4E + 08    14           2.2E + 08______________________________________ .sup.1 Cultures grown in basal salts liquid medium with vitamins and 80 g glucose/L. .sup.2 Blastospores collected from 4day old cultures. .sup.3 Viabllity determined by 6hour germination assay in potato dextrose broth for airdried blastospores. .sup.4 Not done. Too few spores were produced to conduct airdrying. .sup.5 Fisher&#39;s protected last significant difference. (P ≧0.05) 
    
     As shown in FIG. 1 and FIG. 2A and B, sporulation by cultures of Paecilomyces fumosoroseus 4491 in MS medium occurred rapidly and prior to glucose or amino acid exhaustion although Casamino acids were being rapidly utilized during days three and four when maximum sporulation was occurring. Paecilomyces fumosoroseus 4491 spore yields reached a maximum concentration, 3.4 to 6.8×10 8  spores/mL, after 4 days growth. FIG. 2A and 2B together depict the substrate utilization pattern of Paecilomyces fumosoroseus in MS medium. Specifically, FIG. 2A shows that MS medium contains excess carbohydrate and FIG. 2B shows that while Casamino acids were essentially depleted after 4 days growth, more than 70 g glucose/L remained (FIG. 2A). Amino acids, therefore, appear to be preferentially used by Paecilomyces fumosoroseus 4491 as a carbon and nitrogen source. 
     These results suggest that past reports on the instability of Paecilomyces fumosoroseus spores were due to spore formation under suboptimal nutritional conditions. By providing liquid grown Paecilomyces fumosoroseus cultures with the nutritional environment outlined herein, high concentrations of desiccation tolerant spores can be rapidly produced. 
     Comparison of the Ability of Various Strains of Paecilomyces fumosoroseus to Produce Desiccation Resistant Spores 
     The ability of MS medium to support rapid and high volume sporulation of desiccation resistant spores is clearly not strain specific. 
     A comparison of 24 Paecilomyces fumosoroseus strains showed that MS medium supported the rapid production of high concentrations of desiccation tolerant spores (Table 1). Analysis of variance indicated that spore yield in all but three of the strains tested was not significantly different and that the total number and percentage of spores surviving freeze-drying were not significantly different for any of the strains tested. 
     Plate-counts were used to measure the viability of spores freeze-dried for storage while 6 hour germination assays in potato dextrose broth were used to assess the viability of air-dried spores and freeze-dried spores produced while screening the 24 different Paecilomyces fumosoroseus strains. A comparison of the 6 hour germination assay and plate count methods showed no significant differences in viability when comparing recently dried spore preparations (data not shown). Difficulties in plating air-dried spore-diatomaceous earth preparations made the 6-hour germination assay the method of choice for these preparations. 
     Air-dried preparations were stored in sealed plastic bags and freeze-dried spore preparations were stored in vacuum sealed ampules at either 4° C. or 22° C. After 5 months storage at 4° C., over 68% of the freeze-dried, vacuum sealed spores remained viable. Liquid culture produced spores air-dried at a relative humidity of 75% maintained 40% viability after 3 months storage at 4° C (FIG. 3). 
     The following examples are presented to describe preferred embodiments and utilities of the present invention and are not meant to limit the present invention unless otherwise stated in the claims appended hereto. For instance, although a majority of experiments involving the production of a high volume of desiccation resistant spores were performed utilizing Paecilomyces fumosoroseus, the medium and methods of the present invention will likely enhance sporulation and desiccation resistance for a variety of similar fungal species. Work with other fungi that are potential biological control agents, such as Colletotrichum gloeosporioides and Fusarium moniliforme have demonstrated that this medium can support rapid liquid culture sporulation. Other entomopathogenic fungi like Paecilomyces fumosoroseus which produce similar liquid culture spores will likely respond to this medium. 
     EXAMPLE 1: Strains and Culture Conditions 
     Paecilomyces fumosoroseus strains were obtained from various locations. Table 1 lists the various strains and their origin. Stock cultures were grown as single spore isolates on potato dextrose agar (PDA), cut into 1 mm 2  agar plugs and stored in 10% glycerol at -80° C. Conidial inocula were produced by inoculating PDA plates with conidial suspension from frozen stock cultures. Submerged cultures were inoculated with conidia from rinsed PDA plates to achieve a final concentration of 5×10 4  conidia/mL. Spore concentrations were determined microscopically with a hemocytometer. Liquid cultures were grown at 28° C. and 300 rpm in a rotary shaker incubator (100 mL in 250 mL baffled flasks). Replicate flasks were used for all treatments and all experiments were repeated at least twice. 
     EXAMPLE 2: Media Compositions 
     Media with various carbon sources, carbon concentrations, carbon-to-nitrogen (CN) ratios, and nitrogen sources were tested for their impact on Paecilomyces fumosoroseus spore yield and stability. The basal component of all medium tested contained per liter: KH 2  PO 4 , 2.0 g; CaCl 2  --2H 2  O, 0.4 g; MgSO 4  --7H 2  O, 0.3 g; CoCl 2  --6H 2  O, 37 mg; FeSO 4  --7H 2  O, 50 mg; MnSO 4  --H 2  O, 16 mg; ZnSO 4  --7H 2  O, 14 mg; thiamin, riboflavin, pantothenate, niacin, pyridoxamine, thiotic acid, 500 μg each; folic acid, biotin, vitamin B 12 , 50 μg each. All medium had an initial pH of 5.5 and pH was uncontrolled during culture growth. The various carbon sources tested were autoclaved separately. The medium tested contained various carbon and nitrogen sources at differing concentrations as noted in the respective tables, graphs, and text. 
     EXAMPLE 3: Substrate Utilization 
     High performance liquid chromatography was used to measure glucose concentrations in culture supernatants, as previously described (Jackson, Slininger &amp; Bothast, 1989). The concentration of 15 amino acids was measured in culture supernatants as o-phthalaldehyde derivatives using reverse-phase HPLC. These amino acids were aspartic acid, glutamic acid, serine, histidine, glycine, threonine, arginine, alanine, tyrosine, methionine, valine, phenylalanine, isoleucine, leucine, and lysine. The sum of the concentrations of the 15 amino acids was used as an approximation for the amino acid concentration in the culture supernatant. 
     EXAMPLE 4: Drying and Storage Studies 
     Liquid culture produced Paecilomyces fumosoroseus spores were dried using two methods: air-drying and freeze-drying. A high percentage of Paecilomyces fumosoroseus spores produced in MS medium survived air-drying (79±12.4%) and freeze-drying (86±10.6%). Statistical analyses of these results showed no significant differences in initial survival after air-drying or freeze-drying for Paecilomyces fumosoroseus 4491 spores produced in MS medium. In air-drying experiments, whole cultures were harvested after 3 days growth and mixed with 5% (w/v) diatomaceous earth (HYFLO, Celite Corp.). In subsequent air drying and freeze drying experiments where stability during storage and biocontrol efficacy were being evaluated, spores were separated from the mycelia by passing the culture through a double layer of cheesecloth twice. Air-drying experiments involved mixing the conidial suspension with 5% diatomaceous earth, filtering off the excess liquid, and drying the filter cake in a biological containment hood (20-30% RH) overnight to 1-5% moisture. Studies which evaluated the impact of the relative humidity (RH) of the drying air on spore survival were performed in a humidity controlled plant growth chamber at 25° C. For storage studies, air-dried spore preparations were kept in plastic bags at temperatures of 4° C. The viability of air-dried Paecilomyces fumosoroseus spores was assessed by adding dried spores to potato dextrose broth and measuring one hundred spores for germ tube formation after 6 hours incubation at 28° C. and 300 rpm in a rotary shaker incubator. 
     For freeze-drying experiments, spore suspensions were mixed (1:1) with a solution containing 20% lactose and 2% bovine serum albumin (BSA) to produce a spore mixture in 10% lactose, 1% BSA. Freeze-drying was performed in a tray dryer (Durastop-MP, FTS Systems) using an automatic-eutectic drying program. This program determined the eutectic point of the sample and set drying conditions based on this information, monitored the primary and secondary drying process, and determined when the drying process was completed. Ten milliliter vials containing 2 mL spore suspensions were used in all studies. At the end of the freeze-drying cycle, vials were sealed under vacuum and stored at 4° C. or 22° C. The viability of freeze-dried spores was assessed in two ways. For long-term storage studies, spore survival was measured by plate counts on potato dextrose agar incubated at 28° C. Prior to plating, freeze-dried spores were rehydrated for one hour at room temperature and diluted with sterile 0.004% phosephaste buffer. When screening various Paecilomyces fumosoroseus strains for spore production and stability after drying, the viability of freeze-dried spores was assessed by the 6 hour germination method previously described for air-dried spores. 
     EXAMPLE 5: Bioassays 
     Biocontrol efficacy studies against B. tabaci were performed with air-dried, liquid culture produced spores of Paecilomyces fumosoroseus ARSEF 4491. Various concentrations of air-dried spore:diatomaceous earth preparations were mixed with water and applied to whitefly-infested hibiscus leaves with a tower sprayer. Solid substrate produced aerial conidia of Paecilomyces fumosoroseus ARSEF 3699 and of Beauveria bassiana ARSEF 252 were used as controls in each experiment. An additional control of diatomaceous earth mixed with spent medium and dried in the same manner as the spore suspensions, was also used in all experiments. Conidial suspensions were sprayed onto hibiscus leaf discs infested with B. tabaci pupae and water agar plates. After spraying, the leaf discs were incubated in moist petri plates. The number of viable Paecilomyces fumosoroseus spores sprayed per mm 3  were measured on water agar plates after 24 hours incubation. Mortality in B. tabaci pupae and adults was assessed. The LD 50  (conidia/mm 2 ) and the potency ratio (LD 50  B. bassiana/LD 50  Paecilomyces fumosoroseus) was used to evaluate biocontrol efficacy of the air-dried liquid culture produced spores and the plate-derived aerial conidia. Under the conditions of this assay, air-dried, liquid culture product Paecilomyces fumosoroseus spores incited significant disease in B. tabaci nymphs (Table 6). These air-dried Paecilomyces fumosoroseus spores had potency ratios (LD 50  Beauveria bassiana: LD 50  Paecilomyces fumosoroseus) which were 8 times higher than solid-substrate produced aerial conidia of Paecilomyces fumosoroseus 4491 and were 4 times higher than the B. bassiana ARSEF 252 standard strain (Table 6). 
     
                       TABLE 6______________________________________Efficacy of Air-dried Spores of  Paecilomyces fumosoroseus for Controlling  Sweetpotato Whitefly (Bemisia tabaci)                Potency Ratio  LD.sub.50 (LD.sub.50 Beauveria bassiana)  (spores/mm.sup.2) (LD.sub.50 Paecilomyces fumosoroseus)______________________________________Control   172.9      0.54  Aerial conidia  Liquid culture 56.6 4.11  Spores 115.6 3.77  Test 1  Test 2______________________________________ 
    
     The improvement in biocontrol efficacy of Paecilomyces fumosoroseus spores compared to Paecilomyces fumosoroseus conidia and B. bassiana conidia was dramatic. Hegedus et al., 1992, showed that spore preparations of B. bassiana were more infective than aerial conidia on the migratory grasshopper, Melanoplus sanguinipes. Conversely, another study suggested that the hydrophobic nature of B. bassiana conidia increased the adherence of these propagules to the cuticle of the green leafhopper, Nephotettix virescens, and significantly improved the biocontrol efficacy of conidia compared to B. bassiana spores (Lane, Trinci and Gillespie, 1991). It is possible that the hydrophobicity issue is less important when dealing with sessile B. tabaci nymphs rather than mobile insects. The rapid germination rate of liquid culture produced spores compared to aerial conidia may have enhanced the efficacy of these propagules in infecting and killing B. tabaci nymphs. 
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