Diagnosis of Enterocytozoon bieneusi by PCR in Stool Samples Eluted from Filter Paper Disks

doi:10.1128/CDLI.7.3.504-506.2000

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Clinical and Diagnostic Laboratory Immunology, May 2000, p. 504-506, Vol. 7, No. 3
1071-412X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Diagnosis of Enterocytozoon bieneusi by PCR in Stool Samples Eluted from Filter Paper Disks

Silvana Carnevale,^* Jorge N. Velásquez, Jorge H. Labbé, Agustín Chertcoff, Marta G. Cabrera, and Mónica I. Rodríguez

Departamento de Parasitología, Instituto Nacional de Microbiología "Dr. Carlos G. Malbrán," and Hospital Municipal de Infecciosas "Dr. Francisco J. Muñiz," Buenos Aires, Argentina

Received 2 November 1999/Returned for modification 7 January 2000/Accepted 3 February 2000

	ABSTRACT

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We report a PCR-based assay for the detection of Enterocytozoon bieneusi. We extracted DNA from feces which had been appliedto filter paper disks and evaluated four preserving solutions.Infected specimens were identified by electrophoresis of ampliconsfrom concentrated formalin-fixed samples and unconcentrated freshfeces. Our findings demonstrate that this methodology is effectivefor sample collection, mailing, and diagnosis of thispathogen.

	TEXT

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The microsporidian species Enterocytozoon bieneusi and Encephalitozoon intestinalis have been associated with chronic diarrheaand wasting in human immunodeficiency virus-infected patients(2, 12, 40). Diagnosis of gastrointestinal micro sporidiosisdepends on direct visualization of spores in stained fecal samplesand species differentiation by transmission electron microscopy(6, 40, 41). Identification to the species level is clinicallyof great value because of the differences in therapy response(1, 13, 26). Most studies involve the use of PCR for detectionof E. bieneusi in fresh or formalin-fixed stool specimens (4,7, 8, 9, 14, 15, 17-20, 28, 29, 33, 37, 38).

Epidemiological investigation of microsporidia has been limited by difficulties in the preservation and transport of fecesand diagnostic methods applied to them. Samples collected on afilter paper are a valuable source of DNA for amplification-basedmethods and may provide a practical solution to many of theseproblems (3, 21, 30).

The purpose of this study was to describe a PCR assay for E. bieneusi employing stool samples collected in different preservingsolutions as impregnated filter paper disks(FPD).

Stool samples and intestinal biopsy specimens were obtained from three human immunodeficiency virus-infected patients withchronic diarrhea and microsporidiosis caused by E. bieneusi. Microsporidialinfections were diagnosed using multiple formalinized stool specimensby light-microscopic examination of samples stained accordingto Weber's modified trichrome method (40) and the quick-hotGram-chromotrope technique (27). Five biopsy specimens fromeach patient were obtained from the distal duodenum by flexiblefiber-optic endoscopy. Two specimens were fixed in 10% formalinfor routine histology and were stained with Giemsa and hematoxylin-eosin.Two other specimens were processed for transmission electron microscopy(11, 31) to confirm E. bieneusi infections. The fifth biopsyspecimen was stored in saline solution at $-$ 20°C for DNA purification.Stool samples were collected in four solutions: (i) 5% formaldehyde(volume ratio of stool to formalin, 1:3), (ii) 0.05% saline solution,(iii) 2.5% potassium dichromate, and (iv) Merthiolate-formalin(MF) (36) (volume ratio of stool to each of these three solutions,1:2). FPD (Whatman no. 1) 1 cm in diameter were used to storethe fecal specimens. After homogenization, samples were spottedon the FPD in two different forms: as suspensions of homogeneousmaterial and as centrifugation pellets following ethyl ether extraction(34). For pellet spotting, samples were resuspended in the remainingsolution and 100 µl was pipetted onto each disk. The FPD wereair dried and stored in individual plastic bags at 4°C for atleast 6months.

Each FPD was incubated for 2 h at 56°C in 500 µl of lysis buffer (100 mM Tris-HCl [pH 8.0], 100 mM EDTA [pH 8.0], 2% sodiumdodecyl sulfate, 150 mM NaCl, and 200 µg of proteinase K/ml).The DNA was purified by phenol-chloroform extractions and precipitationwith absolute ethanol and was resuspended in 10 µl of sterileredistilledwater.

The primers Eb.gc (5'-TCAGTTTTGGGTGTGGTATCGG-3') and Eb.gt (5'-GCTACCCATACACACATCATTC-3') (38) were used to amplify a 210-bpfragment of the unique rRNA intergenic spacer sequence of E. bieneusi(GenBank accession no. L20290) (43). All PCRs were carriedout as previously described (38). Five microliters of DNA purifiedfrom each FPD was employed in this assay. The amplification procedureincluded 30 s of denaturation at 98°C in the first cycle (94°Cafterwards) followed by 30 s of annealing at 49°C and 90 s ofextension at 72°C for 36 cycles. After the first PCR, 10 µl ofamplified material was used to run a second PCR under the sameconditions and with the same primers as the first PCR. The amplifiedmaterial (20 µl) was fractionated by 1.5% agarose gel electrophoresisand visualized by ethidium bromide staining. After the first roundof PCR amplification, the analysis was performed on 12.5% polyacrylamidegels (22) followed by silver staining (PlusOne DNA silver stainkit; Pharmacia, Uppsala,Sweden).

The first round of PCR produced the expected DNA fragments on ethidium bromide- and silver-stained gels when DNA from concentratedfresh feces on FPD was used as a template (Fig. 1A). No bandswere detected when DNA from uncentrifuged stool samples or specimenscollected in preservative solutions was used. A second round ofPCR resulted in efficient amplification of all non-formalin-fixedspecimens, independent of the method used to apply feces to themembrane (Fig. 1B, lanes 1 to 4). Higher amounts of product fromconcentrated samples than from those placed on FPD as suspensionswere observed for both fresh feces and potassium dichromate-preservedspecimens. Amplicons of 210 bp could also be detected in the secondround of PCR amplification using DNA prepared from formalin-fixedsamples that had been ethyl ether extracted before FPD spotting(Fig. 1B, lane 6). No PCR products from nonconcentrated fixedspecimens could be observed (Fig. 1B, lane 5). The same resultswere obtained with templates from samples collected in MF solution(Fig. 1B, lanes 7 and 8). Silver staining did not improve theresults of the second PCR assay (data not shown). All resultswere identical for samples obtained from the three studied patients.DNA purified from frozen biopsy specimens of an E. bieneusi-infectedpatient was used as a positive control. DNA from duodenal biopsyspecimens from known E. bieneusi-negative individuals was employedas a negative control in all assays.

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FIG. 1. Agarose gel electrophoresis (ethidium bromide stain) of PCR products. (A) First round of amplification; (B) double PCR amplification. Lanes 1 and 2, fresh sample; lanes 3 and 4, specimen in 2.5% potassium dichromate solution; lanes 5 and 6, formalin-fixed sample; lanes 7 and 8, specimen preserved in MF. Lanes 1, 3, 5, and 7, homogeneous suspension; lanes 2, 4, 6, and 8, concentrated sample. Lanes 9 and 10, positive and negative controls, respectively; lane 11, reaction mixture; lane M, 100-bp ladder.

The epidemiology of E. bieneusi infection has not been completely elucidated, and more information is needed on clinical featuresin HIV-infected patients and in other hosts, the impact of antiretroviraltreatment, and geographical, environmental, and seasonal factors(5, 23, 40). Several PCR protocols for E. bieneusi haveused fresh stool samples that were frozen or stored and transportedat ambient temperatures for immediate processing (10, 32,33, 37). Field conditions may limit the handling, transport,and refrigeration of the specimens. Other investigators have employedformalin-fixed fecal specimens, which can be transported and stored,but at present there is no information on the use of other fixativesfor fecal specimens to be tested by microsporidial PCR protocols(4, 9, 14, 29).

In our study, examination of products after the first round of PCR showed good amplification with DNA from centrifuged freshfeces spotted on FPD. Although some authors used different proceduresto remove PCR inhibitors (15, 25, 36, 42), our resultsdemonstrated that such removal was unnecessary with stool sampleseluted from FPD. Negative results observed with preserved specimensshowed a low level of DNA recovery. When fecal specimens are preservedin formalin, it is very difficult to amplify the DNA of microsporidialspores because this fixative reacts with the DNA (14). Thispossibility may be considered for the other fixatives employed(14, 16).

Our findings clearly show the advantage of our double PCR method and confirm that different preserved or fresh specimens canbe employed with good diagnostic results. The filter paper specimensfacilitate collection, transport, and storage because they havelittle weight, are cost effective, require minimal storage space,and maintain stable DNA during long periods (3, 24, 39).This study extends the diagnostic possibilities to laboratoriesemploying all the usual collection procedures. Moreover, positiveresults obtained with unconcentrated fresh samples and the useof FPD as specimen support add great value to this technique becausefecal specimens may be collected by untrained persons and mailedto a central diagnostic laboratory foridentification.

	ACKNOWLEDGMENTS

We express our appreciation to colleagues who advised and assisted with the study: José M. Peralta, from the Instituto deMicrobiologia, CCS, Universidade Federal de Rio de Janeiro, Riode Janeiro, Brazil; Raúl Franco, from the Departamento de Bacteriología,Instituto Nacional de Microbiología "Dr. Carlos G. Malbrán,"Buenos Aires, Argentina, and Fernando Sodré, from the UniversidadeFederal Fluminense, Niteroi,Brazil.

	FOOTNOTES

^* Corresponding author. Mailing address: Lituania 520, (1826) Remedios de Escalada, Buenos Aires, Argentina. Phone: 54 11 42420883. Fax: 54 11 4301 7437. E-mail: jorsil{at}overnet.com.ar.

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2. Cali, A., D. P. Kotler, and J. M. Orenstein. 1993. Septata intestinalis n.g., n.sp., an intestinal microsporidian associated with chronic diarrhea and dissemination in AIDS patients. J. Eukaryot. Microbiol. 40:101-112[Medline].

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1.	Blanshard, C., D. S. Ellis, D. G. Tovey, S. Dowell, and B. G. Gazzard. 1992. Treatment of intestinal microsporidiosis with albendazole in patients with AIDS. AIDS 6:311-313[Medline].
2.	Cali, A., D. P. Kotler, and J. M. Orenstein. 1993. Septata intestinalis n.g., n.sp., an intestinal microsporidian associated with chronic diarrhea and dissemination in AIDS patients. J. Eukaryot. Microbiol. 40:101-112[Medline].
3.	Carducci, C., L. Ellul, I. Antonozzi, and A. Pontecorvi. 1992. DNA elution and amplification by polymerase chain reaction from dried blood spots. BioTechniques 13:735-737[Medline].
4.	Carville, A., K. Mansfield, G. Widmer, A. Lackner, D. Kotler, P. Wiest, T. Gumbo, S. Sarbah, and S. Tzipori. 1997. Development and application of genetic probes for detection of Enterocytozoon bieneusi in formalin-fixed stools and in intestinal biopsy specimens from infected patients. Clin. Diagn. Lab. Immunol. 4:405-408[Abstract].
5.	Conteas, C. N., G. W. Berlin, C. E. Speck, S. S. Pandhumas, M. J. Lariviere, and C. Fu. 1998. Modification of the clinical course of intestinal microsporidiosis in acquired immunodeficiency syndrome patients by immune status and anti-human immunodeficiency virus therapy. Am. J. Trop. Med. Hyg. 58:555-558[Abstract].
6.	Conteas, C. N., T. Sowerby, G. W. Berlin, C. E. Speck, S. S. Pandhumas, M. J. Lariviere, and C. Fu. 1996. Fluorescence techniques for diagnosing intestinal microsporidiosis in stool, enteric fluid, and biopsy specimens from acquired immunodeficiency syndrome patients with chronic diarrhea. Arch. Pathol. Lab. Med. 120:847-853[Medline].
7.	Coyle, C. M., M. Wittner, D. P. Kotler, C. Noyer, J. M. Orenstein, H. B. Tanowitz, and L. M. Weiss. 1996. Prevalence of microsporidiosis due to Enterocytozoon bieneusi and Encephalitozoon (Septata) intestinalis among patients with AIDS-related diarrhea: determination by polymerase chain reaction to the microsporidian small-subunit rRNA gene. Clin. Infect. Dis. 23:1002-1006[Medline].
8.	da Silva, A. J., D. A. Schwartz, G. S. Visvesvara, H. de Moura, S. B. Slemenda, and N. J. Pieniazek. 1996. Sensitive PCR diagnosis of infections by Enterocytozoon bieneusi (microsporidia) using primers based on the region coding for small-subunit rRNA. J. Clin. Microbiol. 34:986-987[Abstract].
9.	da Silva, A. J., F. J. Bornay-Llinares, C. del Aguila de la Puente, H. Moura, J. M. Peralta, I. Sobottka, D. A. Schwartz, G. S. Visvesvara, S. B. Slemenda, and N. J. Pieniazek. 1997. Diagnosis of Enterocytozoon bieneusi (microsporidia) infections by polymerase chain reactions in stool samples using primers based on the region coding for small-subunit ribosomal RNA. Arch. Pathol. Lab. Med. 121:874-879[Medline].
10.	del Aguila, C., R. Navajas, D. Gurbindo, J. T. Ramos, M. J. Mellado, S. Fenoy, M. A. Muñoz Fernandez, M. Subirats, J. Ruiz, and N. J. Pieniazek. 1997. Microsporidiosis in HIV-positive children in Madrid (Spain). J. Eukaryot. Microbiol. 44:845-855.
11.	Desportes, I., I. Hilmarsdottir, C. Romaña, S. Tanguy, A. Datry, and M. Gentilini. 1991. Characteristics of the microsporidian Enterocytozoon bieneusi: a consequence of its development within short-living enterocytes. J. Protozool. 38:111-113.
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