Spore shedding pattern of Enterocytozoon bieneusi in asymptomatic children

doi:10.1099/jmm.0.45832-0

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Spore shedding pattern of Enterocytozoon bieneusi in asymptomatic children

Mathirut Mungthin¹, Ittisak Subrungruang², Tawee Naaglor¹, Pote Aimpun³, Wirote Areekul³ and Saovanee Leelayoova¹

^1,3Department of Parasitology¹ and Department of Military and Community Medicine³, Phramongkutklao College of Medicine, 315 Ratchawithi Rd, Ratchathewi, Bangkok 10400, Thailand ²Department of Protozoology, Faculty of Tropical Medicine, Mahidol University, Bangkok, Thailand

Correspondence Mathirut Mungthin mathirut{at}pmk.ac.th

Received July 22, 2004
Accepted January 13, 2005

Stool samples from seven human immunodeficiency virus (HIV)-negativeand two HIV-positive children with asymptomatic Enterocytozoonbieneusi infections were daily examined to quantify spore sheddingusing Gram-chromotrope staining under light microscopy. Thespore shedding pattern and intensity in these children was variable.Mean spore concentrations in the stool samples from these childrenranged from 2.4 x 10² to 1.2 x 10⁵ spores per gram. Light microscopycould detect spores in stool specimens for 9–33 days,while PCR was able to detect E. bieneusi in stool specimensfor 3–40 days longer. This suggests that light microscopymay not detect low levels of spore shedding. Considering thatthe asymptomatic group are a potential source of infection,detection methods with a higher sensitivity should be used.

Abbreviation: HIV, human immunodeficiency virus.

INTRODUCTION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Enterocytozoon bieneusi is one of the common causes of chronicdiarrhoea in AIDS patients, especially in those with CD4⁺ cellcounts less than 100 mm^–3 (Weber et al., 1994; Kotler & Orenstein, 1998;Franzen & Müller, 2001). E.bieneusi can also cause diarrhoea in patients with other immunosuppressiveconditions such as organ transplantation (Gumbo et al., 1999a),and in immunocompetent hosts (Sandfort et al., 1994; Sobottka et al., 1995).

It is assumed that these organisms are transmitted via the faecal-oralroute since their spores are shed via stools. Possible modesof transmission, including human-to- human (Hutin et al., 1998;Gumbo et al., 1999b), animal-to-human (Dengjel et al., 2001;Sadler et al., 2002; Sulaiman et al., 2003) and waterborne transmission(Hutin et al., 1998; Dowd et al., 1998; Fournier et al., 2000),have been suggested in several studies. The role of human-to-humantransmission of intestinal microsporidiosis was indicated ina case-control study which showed that homosexuality was oneof the risk factors of intestinal microsporidiosis (Hutin et al., 1998).A study of E. bieneusi infection in human immunodeficiencyvirus (HIV)-positive patients in Zimbabwe also showed that thosewho had a history of contact with a diarrhoeal patient had a1.9-fold greater risk of getting the infection (Gumbo et al., 1999b).Considering this mode of transmission, humans are theimportant source of this organism.

Variation of spore shedding intensity of E. bieneusi in HIV-positivepatients was shown in two recent studies (Clarridge et al., 1996;Goodgame et al., 1999). However, to our knowledge therehave been no reports on the spore shedding pattern of E. bieneusiin asymptomatic cases, the potential source of the infection.Therefore we aimed to study the pattern of E. bieneusi sporeshedding in asymptomatic children.

METHODS

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Stool specimens were collected from seven HIV-negative and twoHIV-positive children with asymptomatic E. bieneusi infectionswho lived at an orphanage in Bangkok, Thailand. The surveysof E. bieneusi infection in these children were conducted betweenOctober 2001 and October 2002. The study was approved by theEthics Committee of the Royal Thai Army Medical Department.

Screening for microsporidial spores in stool specimens was performedby Gram-chromotrope staining (Moura et al., 1996). Species-specificPCR was used for the identification of E. bieneusi (Katzwinkel-Wladarsch et al., 1996).Stool examination was performed daily until negativefor E. bieneusi by Gram-chromotrope staining for 2 months.

A quantitative assay for E. bieneusi spores was performed usinglight microscopy. After vigorous mixing of each stool specimen,0.2 g of stool sample was diluted in 600 µl of PBS. Thediluted sample was then thoroughly agitated until a completelyhomogeneous suspension was achieved. Ten microlitres of eachdiluted stool specimen was smeared onto a slide for Gram-chromotropestaining. Three slides were made for each specimen. E. bieneusispores were defined as violet oval structures of 1–2 µmwith vacuole or band as described previously (Moura et al., 1996).Slides were examined at a magnification of x100 withoil immersion for the whole smear by an experienced microscopist.For each specimen the mean of the counted spores from the threeslides was calculated as spores per gram to represent the amountof spores in the specimen.

Stool specimens that were negative when examined by light microscopewere processed for PCR detection of E. bieneusi. Extractionof genomic DNA was performed by using the QIAamp DNA Stool MiniKit (QIAGEN) following the manufacturer's instructions. GenomicDNA of each sample was kept at –20 °C until use. PCRamplification was performed using the primer pair (MSP3 andMSP4B) to amplify a 508 bp fragment of E. bieneusi, containing122 bp of the 3' end of the small-subunit rRNA gene, 243 bpof the intergenic transcribed spacer and 143 bp of the 5' regionof the large-subunit rRNA gene, with the conditions as describedby Katzwinkel-Wladarsch et al. (1996). The PCR products andmolecular markers were electrophoresed in 2 % agarose gel (FMCBioproducts) with 1.5 % Tris/borate/EDTA (TBE) buffer usinga gel electrophoresis device (Bio-Rad). Bands were visualizedafter staining with ethidium bromide under UV light and documentedon high-density printing paper using the UVsave gel documentationsystem I (Uvitech).

RESULTS AND DISCUSSION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

The spore shedding pattern of E. bieneusi was examined in sevenHIV-negative and two HIV-positive children aged between 9 and23 months. The two HIV-positive children were on zidovudine(AZT) and didanosine (ddI) treatment; unfortunately we haveno record of their CD4 lymphocyte count. Four of the childrenwere girls and five were boys. None of them had diarrhoeal symptomsduring the study.

The number of stools collected from each child is shown in Table 1.During the period in which spores could be detected by lightmicroscopy, the percentage of days on which stool samples weresuccessfully collected from each child varied between 33 and100. After a negative result by light microscopy, stool specimenswere collected daily for 2 months, with the response rate between55 and 95 %. According to the childcare workers, the main reasonsfor missing specimens were that the children did not pass astool or the childcare workers could not collect the specimensbecause they were too small to collect. The spore counts ofthree slides per specimen showed a little variation. Fig. 1shows the mean concentration of spores per gram of stool, whichranged from 2.4 x 10² to 1.2 x 10⁵ spores per gram. The twoHIV-positive children excreted mean spore concentrations of2.5 x 10⁴ and 3.4 x 10³ spores per gram. The maximal spore concentrationreached 5.7 x 10⁵ spores per gram in one child who was HIV-negative.Quantitative spore counting by Goodgame et al. (1999) showedspore concentrations ranging from 4.5 x 10⁵ to 4.4 x 10⁸ sporesper gram in stool specimens of 20 patients. They also showedthat the quantity of spores excreted in the stool and the intensityof the infection examined by tissue biopsy were well correlated.In comparison, the specimens from asymptomatic HIV-positiveand -negative children in the present study contained lowerspore concentrations, ranging from 2.4 x 10² to 1.2 x 10⁵ sporesper gram. However, the intensity of infection alone may notbe enough to explain the different clinical outcomes in E. bieneusiinfection.

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Table 1. Duration of E. bieneusi spore shedding in each child as detected by light microscopy and PCR

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Fig. 1. Concentrations of E. bieneusi spores in stool specimens of nine children. For each child the graph shows the maximum and minimum values recorded and the mean.

The amount of oocyst excretion in stools has been shown to becorrelated with the clinical outcomes in cases of cryptosporidiosis.The study of Cryptosporidium oocyst excretion patterns in healthyvolunteers showed that those who had diarrhoeal illness excreted50-fold more oocysts than those who had mild enteric symptomsor no symptoms (Chappell et al., 1996). However, AIDS patientswith diarrhoeal illness caused by Cryptosporidium parvum mightexcrete both low and high numbers of oocysts (Goodgame et al., 1993).A study of the spore shedding pattern of E. bieneusiin HIV-positive patients also showed the same picture. Semi-quantitativeexamination of stool specimens from 23 HIV-positive patientsby Clarridge et al. (1993) showed no correlation between thenumbers of spores shed and diarrhoeal patterns. In another study,it was also shown that the intensity of spores in stool specimenswas not correlated to the 24-hour stool volume (Goodgame et al., 1999).This might indicate that factors other than theintensity of infection contribute to symptoms. Thus, the relationshipbetween the intensity and clinical outcomes of the infectionshould be further studied in different groups of patients includingimmunocompetent and immunocompromised patients with differentclinical manifestations.

Marked variation of E. bieneusi spore intensity occured in eachstool specimen from each child, as shown in Fig. 2. Stool-to-stoolvariability of spore shedding showed 7- to 411-fold differencesin each child. Thus it appears that spore production is nota constant process. The number of spores shed tended to decreaseafter a period of time. This might indicate the spontaneouscessation of infection in these children.

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Fig. 2. Variation of E. bieneusi spore concentration in stool specimens from nine children. Only specimens that could be quantified by light microscope are plotted. Open and solid symbols represent HIV-positive and HIV-negative cases, respectively.

The length of time over which spores could be detected by lightmicroscopy for each child was measured as the number of daysfrom the first day of spore detection to the last day of positivespore detected, and ranged between 9 and 33 days. However, duringthis time, not all specimens were positive for E. bieneusi bylight microscopy. In one child, only 25 % of the stained smearsgave positive results when examined by an experienced microscopist;the period between two positive stool specimens was from 1 dayto 2 weeks. Using a PCR method for the detection of E. bieneusi,all the Gram-chromotrope-negative stool specimens that occurredin-between Gram-chromotrope-positive ones showed a positivespecific band. PCR was also used to detect E. bieneusi in thenegative stool specimens collected after the duration of E.bieneusi positivity by light microscopy.

Table 1 shows the duration of E. bieneusi-positive PCR, whichcould detect E. bieneusi in the stool specimens for 3–40days longer. The lowest spore concentration detected by lightmicroscopy was approximately 3 x 10² spores per gram. This mightreflect the sensitivity of light microscopy for the detectionof E. bieneusi spores in stool specimens. PCR could detect E.bieneusi in the Gram-chromotrope-negative stool specimens duringand after the duration of E. bieneusi positivity by light microscopy.Low sensitivity of light microscopy has been shown in severalstudies (Rinder et al., 1998; Menotti et al., 2003). A multicentrestudy showed that PCR detected as little as 10² spores per gramwhile a detection limit of 10⁴ spores per gram of stool wasshown by light microscopy (Rinder et al., 1998). More recently,a real-time PCR method has been developed in order to accuratelyquantify E. bieneusi DNA in stool specimens (Menotti et al., 2003).Real-time PCR showed a much higher sensitivity for thedetection of E. bieneusi spores; it could detect as little as $~$ 40 spores per gram. Light microscopy could detected E. bieneusispore with a sensitivity of $~$ 40 000 spores per gram.

In conclusion, lower E. bieneusi spore concentrations in HIV-positiveand -negative asymptomatic children have been shown comparedto the previous study of HIV-positive patients with intestinalmicrosporidiosis. The spore shedding pattern and intensity inthese children was variable. We found that light microscopymay not detect low levels of spore shedding. Thus, the roleof the asymptomatic group as the source of infection is importantand might be under-rated. Using detection methods with a highsensitivity, such as PCR, should be useful in providing moreepidemiological data. Until we have enough information for thedetermination of prevention and control strategies, in an orphanagewhere E. bieneusi infection could spread easily universal precautionsshould be taken.

ACKNOWLEDGEMENTS

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

This work was supported by Phramongkutklao Research Fund. Wethank the director and childcare workers of this orphanage whokindly supported this study.

REFERENCES

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

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