Pesticide exposure in honey bees results in increased levels of the gut pathogen Nosema
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Global pollinator declines have been attributed to habitat destruction, pesticide use, and climate change or some combination of these factors, and managed honey bees, Apis mellifera, are part of worldwide pollinator declines. Here we exposed honey bee colonies during three brood generations to sub-lethal doses of a widely used pesticide, imidacloprid, and then subsequently challenged newly emerged bees with the gut parasite, Nosema spp. The pesticide dosages used were below levels demonstrated to cause effects on longevity or foraging in adult honey bees. Nosema infections increased significantly in the bees from pesticide-treated hives when compared to bees from control hives demonstrating an indirect effect of pesticides on pathogen growth in honey bees. We clearly demonstrate an increase in pathogen growth within individual bees reared in colonies exposed to one of the most widely used pesticides worldwide, imidacloprid, at below levels considered harmful to bees. The finding that individual bees with undetectable levels of the target pesticide, after being reared in a sub-lethal pesticide environment within the colony, had higher Nosema is significant. Interactions between pesticides and pathogens could be a major contributor to increased mortality of honey bee colonies, including colony collapse disorder, and other pollinator declines worldwide.
KeywordsApis mellifera Imidacloprid Nosema Sub-lethal Pesticides Pathogens
The honey bee, Apis mellifera, is arguably the most important pollinator of agricultural crops (Klein et al. 2007). While worldwide managed honey bee populations have increased over the last 50 years, colony populations have decreased significantly in many European and North American nations (Aizen and Harder 2009) as a result of habitat destruction, pesticide use, pathogens, and climate change (NRC 2007) or some combination of these factors (vanEngelsdorp and Meixner 2010). At the same time, cultivation of crops that are dependent on insects for pollination (Aizen et al. 2009) has increased. The ability to provide sufficient colonies to meet this anticipated demand is questionable, especially in light of the elevated losses experienced by US beekeepers over the winters of 2006/2007 and 2007/2008 (vanEngelsdorp et al. 2007; vanEngelsdorp et al. 2008). Colonies that die with a condition known as colony collapse disorder (CCD) make up a significant proportion of recent overwintering losses in the USA (vanEngelsdorp et al. 2008). While the cause of CCD remains unknown, affected colonies are often infected with a greater variety and higher loads of disease agents than apparently healthy colonies (Johnson et al. 2009; vanEngelsdorp et al. 2009a; Cox-Foster et al. 2007). This suggests that some factor or combination of factors may be weakening bees by making them more susceptible to infection (vanEngelsdorp et al. 2009a). A myriad of abiotic and biotic factors can adversely affect the ability of honey bees to fight infection, including interactions between disease agents, mite parasitism, poor nutrition, and sub-lethal exposure to pesticides (Johnson et al. 2009; vanEngelsdorp et al. 2009a). Systemic pesticides such as imidacloprid pose a new route of exposure in pollen and nectar and have been demonstrated to have negative effects on learning in adult bees (Decourtye et al. 2004).
Here we test the hypothesis that bees exposed to sub-lethal levels of pesticide are more susceptible to disease. We exposed colonies of honey bees to the insecticide imidacloprid at sub-lethal levels and then challenged newly emerged workers from those colonies with the gut parasite Nosema spp., two species (Nosema apis and Nosema ceranae) of which are known to adversely affect colony health (Higes et al. 2008; Kauko et al. 2003). The pesticide dosages used were below levels demonstrated to cause effects on longevity or foraging in adult honey bees (Maus et al. 2003; Bonmatin et al. 2007; Deseneux et al. 2007).
Materials and methods
For 10 weeks, we continually exposed full sized colonies of bees (30–40,000 adults) to 5 and 20 ppb imidacloprid by provisioning colonies with protein supplement patties spiked with the pesticide. After 5 and 8 weeks of exposure (ca. 1.5 and 2.5 generations of exposure), wax combs with emerging brood were taken into the laboratory and groups of newly emerged adult bees from selected colonies were removed and either used to determine fresh weight or caged and fed a suspension containing spores of the known bee pathogens N. apis and N. ceranae over the first 2 days of adult life. Ten days later, bees were sacrificed and the development of Nosema infection in individual bees determined.
Chronic imidacloprid exposure to colonies
Thirty honey bee colonies were used and divided into three treatment groups of ten colonies each. Colonies were established in April 2008 in five apiaries, approximately 0.5 km apart containing two colonies from each treatment group (total colonies per apiary = 6). Packages of bees (1.8 kg) were installed in new hive equipment including frames with wax-coated plastic foundation. All queens established in study colonies came from the same genetic source. All colonies were managed to limit the levels of other pests and pathogens. All colonies were fed equal amounts of sucrose syrup until natural forage was abundant in May. Treatments consisted of untreated Megabee® protein patties (100 g each) or patties containing 5 and 20 ppb of imidacloprid made by mixing neat material with the sucrose solution used to make the protein patties. Samples were taken of fresh treated protein patties and analyzed for imidacloprid content to insure proper delivery of the target dose. Beginning in May 2008, each colony received four 80-g patties per week for 10 weeks. Unconsumed patties were removed after 7 days, weighed to measure consumption, and replaced with new treatment protein patties. Adult bees and stored pollen “bee bread” were collected 1 week after the 10-week feeding period and analyzed for imidacloprid levels. Samples (>5 g) of newly emerged bees and random-aged bees from each experimental hive and protein patties from each treatment group were all analyzed for imidacloprid levels at the USDA-AMS laboratory in Gastonia, NC, using GC/MS with a limit of detection of 0.1 ppb.
Experimental bees and pathogen challenge
Five weeks into treatment in July 2008, a single brood frame with emerging worker bees were removed from each of three to four colonies treatment and held in an incubator at 34°C overnight. Newly emerged bees were collected the next morning and placed in groups of 30 bees per cage for Nosema challenge. An additional 20 newly emerged bees per colony were weighed to determine average emerged bee weight. A Nosema spore suspension was made by taking the mid-guts of ten workers from a single Nosema-infected colony and macerating the guts in 10 ml of water and determining the total spore count using the methods of Cantwell (1970) and a hemocytometer slide. The spore suspension was then centrifuged for 10 min at 3,000 rpm, the supernatant discarded, and the spore pellet resuspended using a 50:50 volume to volume sucrose solution to reach a final spore concentration of one million spores per milliliter of solution. Ten milliliters of this solution was fed to each cage of 30 bees over the first 2 days of adult life and after complete consumption of the 10 ml each bee received an approximate dose of 333,333 spores over 2 days. Treated bees were allowed to age in cages for 12 days, sacrificed, and spore levels determined for each bee using standard light microscopy and a hemocytometer after the methods of Cantwell (1970). Nosema spore data was log transformed prior to analysis to meet statistical assumptions. Mortality was monitored daily and no cage exceeded 20% over 12 days. At day 12, ten randomly selected live bees were used for spore determination on an individual bee basis. A second trial was conducted in August, 8 weeks into treatment and this time however emerged bees were feed 10 ml of sugar solution containing either 0 (control), 0.1, or 1 million spores per milliliter to explore potential effects of inoculum dose of pathogen growth. The Nosema spore suspension was made using bees from the same source colony as before. Mortality in the cages averaged less than 20% after 12 days. Samples of the Nosema spore suspensions from both dates were analyzed for species composition using established molecular methods (Chen et al. 2008) and found to be predominantly N. ceranae but a weak band corresponding to N. apis was also detected indicating a mixed co-infection of the two species which is still quite common (Chen et al. 2008).
Levels of imidacloprid in bee bread (stored pollen/protein patties) and random-aged worker bees from experimental colonies and average weights of newly emerged bees from the three colony treatments for trials 1 and 2 in July and August 2008, respectively (n = 20 bees/hive)
Imidacloprid levelsa (mean ± SEM, ppb)
Emerged bee weight (mean ± SEM, n = 20 beesd)
Bee bread from coloniesb
Random-aged bees from coloniesb
Imid. level emerged beesc
Emerged bee weight (g) July trial 1
Emerged bee weight (g) Aug. Trial 2
0.20 ± 0.22
0.6 ± 0.31
0.115 ± 0.0014
0.116 ± 0.0018
Low 5 ppb
1.62 ± 0.68
1.58 ± 0.68
0.112 ± 0.0016
0.116 ± 0.0017
High 20 ppb
3.49 ± 1.55
3.67 ± 1.48
*0.106 ± 0.0017
0.116 ± 0.0020
The group of 30 colonies that provided experimental bees for cage experiments were in good health as indicated by low mite and disease levels. Only three of these colonies tested positive for Nosema at the beginning of the trial and those three colonies were excluded from use. At the end of 10 weeks, eight of 30 tested positive for Nosema but there was surprisingly no relationship between Nosema infection and imidacloprid treatment which would have been predicted by the lab study. Three control, three 5 ppb, and two 20 ppb colonies tested Nosema positive, with average spore counts of 4.3, 2.9, and 0.5 million spores per bee, respectively. Varroa mite counts were low with an average mite count of 0.36 mites/100 bees, well below damaging levels which range from five to ten mites per 100 bees, with 27 of 30 colonies testing positive using 300 adult bees (Lee et al. 2010). No colonies tested were found to have tracheal mites.
We clearly demonstrate an interaction between sub-lethal exposure to imidacloprid at the colony level and the spore production in individual bees of honey bee gut parasite Nosema. Two similar studies have just been published that directly treated individual bees with imidacloprid, fipronil, or thiacloprid and then challenged them with Nosema with similar synergistic interaction between Nosema and pesticide exposure (Alaux et al. 2010; Vidau et al. 2011). Our study differs in several significant ways; (1) our study employed sub-lethal colony-level pesticide chronic exposure instead of laboratory direct exposure to experimental bees, (2) no imidacloprid residues could be found in the newly emerged worker bees challenged in our study (Table 1), (3) our test bees could only have received pesticide exposure during larval development, thus (4) pesticide exposure to test bees could only have been indirectly from brood food from nurse bees (Winston 1987) that were exposed as they fed on imidacloprid-spiked protein. We can only speculate as to why sub-lethal exposure in brood food to larva resulted in increased spore production in adult bees. Since Nosema initiates infection in the mid-gut then perhaps in the larval stages the mid-gut ways altered or weakened in some manner that resulted in increased Nosema infection in adult bees. Vidau et al. (2011) failed to demonstrate a change in the pesticide detoxification system in adult bees yet still demonstrated an increase in mortality in adult bees when pesticides and Nosema were combined. Alaux et al. (2010) showed that co-exposure to imidacloprid and Nosema weakened bees but they also showed a trend toward a slight decrease in spore production with pesticide exposure. Individual bees in our study showed a marked increase in Nosema spore production in the laboratory but the parent colonies failed to show increased Nosema levels over time. Our understanding of N. ceranae at the colony level is still very limited as colony-level spore counts can be highly variable. Perhaps spore production is not the proper way to measure N. ceranae infection as has always been the case with N. apis? Taken together these three studies clearly demonstrate synergism between pesticides and Nosema. The current study, with the more robust chronic sub-lethal pesticide exposure at the colony level, clearly demonstrates that such interactions are possible in the real world, not just in a laboratory setting. Additional research is needed to understand the underlying mechanisms of pesticide pathogen interactions. This is especially true in our study in trying to determine how the pesticide moved in the colony, affected nurse bees, and what level of exposure that larvae in these colonies actually received. The pesticide was consumed equally among the two dosages and house bees contained the pesticide but the pharmacokinetics within the colony is yet to be determined.
Past studies have found that chronic, sub-lethal exposure to pesticides can have an adverse effect on colonies (Bendahou et al. 1999) and has been associated with overt disease outbreaks in honey bees (Morse et al. 1965). Conversely, further infection with the chronic bee paralysis virus can affect honey bee tolerance to agricultural pesticides (Bendahou et al. 1997). Recent increases in colony losses in the USA and Europe have drawn particular attention to one relatively new class of systemic pesticides, the neonicotinoids, of which imidacloprid is a member. Beekeeper conviction that imidacloprid is responsible for colony losses in France has resulted in the withdrawal of its registration (under the trade name Gaucho, Bayer, Leverkusen, Germany) as a seed treatment for sunflowers and corn Ministere de l’Agriculture et de la Peche (1999 and 2004). Similar pressure in California has resulted in a reevaluation of four neonicotinoids, including imidacloprid, because of elevated levels of residues in leaves and blossoms of ornamental plants after imidacloprid applications.
The published levels of imidacloprid expressing acute and chronic toxicity on bees are variable and conflicting (Nguyen et al. 2009). Most studies suggest that imidacloprid can cause disorientation and associative learning problems in honey bees at exposure levels above 20 ppb (Decourtye et al. 2004; Deseneux et al. 2007). However, crop residue studies have detected imidacloprid at levels of 2–5 ppb in pollen and >1.5 ppb in nectar of seed-treated corn, sunflowers, and rape (Kauko et al. 2003) well below the 20 ppb level documented to cause acute and chronic toxicity effects. To our knowledge no studies have examined chronic effects of dietary exposure to imidacloprid in functional colonies over multiple brood cycles and potential synergistic effects of pesticide and disease interactions. Our results suggest that the current methods used to evaluate the potential negative effect of pesticides are inadequate. This is not the first study to note a complex and unexpected interaction between low pesticide exposure and pathogen loads. Trematodes levels in amphibian populations are driven by atrazine in the aquatic environment (Rohr et al. 2008). Elevated levels of the fungicide chlorothalonil in honey bees have been associated with “entombed pollen” which is linked with increased risk of colony mortality (vanEngelsdorp et al. 2009b). The call for a reevaluation of pesticide test protocols required for the registration of products is not new (Colin et al. 2004; Halm et al. 2006). These proposed new standards utilize the Predicated No Effect Concentration which is determined using chronic and acute toxicity data and not potentially indirect effects of pesticide exposure, such as increased susceptibility to pathogens. With the wide variety of pesticides that have been documented in failing beehives (Mullen et al. 2010), it is imperative that we understand both the synergistic effects these compound may have and the interactions with other variables, like pathogens, involved in bee health. We suggest new pesticide testing standards be devised that incorporate increased pathogen susceptibility into the test protocols. Lastly, we believe that subtle interactions between pesticides and pathogens, such as demonstrated here, could be a major contributor to increased mortality of honey bee colonies worldwide.
These studies were made possible with the help of Nathan Rice, Vic Levi, Mike Embry, Terry Patton, and Amy Miller. Financial support was provided to JSP from the USDA-ARS Areawide Project to improve bee health and to DVE from the Pennsylvania Department of Agriculture, and GD from the North American Pollinator Protection Campaign and Foundation from the Preservation of Honey Bees.
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- Bendahou N, Bounias M, Fleche C (1997) Acute toxicity of cypermethrin and fenitrothion on honeybees (Apis mellifera mellifera) according to age, formulations and (chronic paralysis virus)/insecticide interaction. J Environ Biol 18:55–65Google Scholar
- Bonmatin JM, Marchand PA, Cotte JF, Aajoud A, Casabianca H et al. (2007) Environmental fate and ecological effects of pesticides. In: delRe AAM, Capri E, Fragoulis G, Trevisan M (eds). 13th Symposium Pesticide Chemistry, Piacenza, Italy, 3–6 September. pp. 827–834Google Scholar
- Cantwell GE (1970) Standard methods for counting Nosema spores. Am Bee J 110:222Google Scholar
- Ministere de l’Agriculture et de la Peche (1999) Avis aux de’ tenteurs et aux utilisateurs de semences de tournesol. J Off Repub Fr. 38Google Scholar
- Ministere de l’Agriculture et de la Peche (2004) Avis aux de’ tenteurs dÕautorisation de mise sur le marche’, aux distributeurs et aux utilisateurs du produit phytopharmaceutique Gaucho. J Off Repub Fr 126Google Scholar
- Kauko L, Honko S, Vartiainen H (2003) Winter mortality and Nosema apis Z. The diagnostic value of Nosema spore counts—a clinical approach. Ann Univ Mariae Curie-Sklodowska Sect DD 58:199–203Google Scholar
- Maus C, Curé G, Schmuck R, Porrini C, Bortolotti L (2003) Safety of imidacloprid seed dressings to honey bees: a comprehensive overview and compilation of the current state of knowledge. Bull Insectol 56:51–57Google Scholar
- Morse RA, Dyce EJ, Gould AC (1965) The treatment of American foulbrood in New York state. Bee World 46:15–17Google Scholar
- National Research Council (2007) Status of pollinators in North America. National Academy of Sciences, Washington, D.C., p 317Google Scholar
- vanEngelsdorp D, Underwood R, Caron D, Hayes J Jr (2007) An estimate of managed colony losses in the winter of 2006-2007: a report commissioned by the Apiary Inspectors of America. Am Bee J 147:599–603Google Scholar
- Vidau C, Diogon M, Aufauvre J, Fontbonne R, Vigues B, Brunet J-L, Texier C, Biron D, Blot N, Alaoui E, Belzunces L, Delbac F (2011) Exposure to sublethal doses of fipronil and thiacloprid highly increases mortality of honeybees previously infected by Nosema ceranae. PLoS One 6(6):e21550. doi: 10.1371/journal.pone.0021550 PubMedCrossRefGoogle Scholar
- Winston M (1987) The biology of the honey bee. Harvard University Press, Cambridge, p 267Google Scholar