Disseminated Mycobacterium lentiflavum Infection in a Human Immunodeficiency Virus-Infected Patient

doi:10.1128/JCM.39.5.2030-2032.2001

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Journal of Clinical Microbiology, May 2001, p. 2030-2032, Vol. 39, No. 5
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.5.2030-2032.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Disseminated Mycobacterium lentiflavum Infection in a Human Immunodeficiency Virus-Infected Patient

S. Ngo Niobe,¹ C. M. Bebear,¹ M. Clerc,¹ J.-L. Pellegrin,² C. Bebear,¹ and J. Maugein¹^,^*

Laboratoire de Bactériologie, Université Victor Segalen Bordeaux 2, 33076 Bordeaux Cedex,¹ and Service de Médecine Interne et Maladies Infectieuses, Hôpital Haut-Lévêque, 33604 Pessac Cedex,² France

Received 6 November 2000/Returned for modification 30 January 2001/Accepted 19 February 2001

	ABSTRACT

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We report the first case of Mycobacterium lentiflavum disseminated infection in a human immunodeficiency virus-infected patient.Conventional identification procedures failed to identify themycobacterial strain, but sequencing of the 16S rRNA gene ledto the species identification. Furthermore, we describe here theanalysis of the 16S-23S rRNA internal transcribed spacer sequenceof M. lentiflavum.

	CASE REPORT

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The patient was a 49-year-old, homosexual male with known human immunodeficiency virus (HIV) seropositivity since 1989. InOctober 1996, he was hospitalized in the Department of InternalMedicine and Infectious Diseases with fever, cough, shortnessof breath, and weight loss. The CD4 count was 40/mm³, and HIV RNA levels were 33,000 copies/ml. A chest computed tomographyscan revealed an interstitial syndrome. Three blood samples forculture were collected on Septi-Chek AFB medium (Roche DiagnosticSystems), and a bronchoalveolar lavage fluid sample was inoculatedonto Löwenstein-Jensen and Colestsos medium slants. After 4 weeks,all the sample cultures grew acid-fast, rod-shaped coccobacilli,subsequently identified as Mycobacterium lentiflavum. The bloodsample isolate, named HL1, was found to be susceptible to clarithromycin(MIC, 1 µg/ml) and rifabutin (MIC, 0.12 µg/ml).

Chemotherapy with three drugs, clarithromycin, rifabutin, and ethambutol, was started. After 4 months of such therapy andthe introduction of a new antiretroviral regimen with two nucleosideanalogs and a protease inhibitor, the patient improved clinicallyand fully recovered for several months. Three blood cultures performedat 3, 6, and 9 months of treatment remained negative. The patientdied 3 years later of cardiacfailure.

Microbiological investigation. Colonies of strain HL1 on Löwenstein-Jensen medium were smooth and 1 to 2 mm in diameter and showed bright yellow pigmentationwith a colony morphology similar to that of M. avium. Subcultureof the isolate showed growth in 4 weeks at 22 and 37°C. For allisolates, conventional identification methods (4) showed negativetests for nicotinic acid production, Tween 80 hydrolysis, nitratereductase, urease, and heat-stable catalase. On the basis of theenzymatic activities the isolate was most closely related to M.avium, but a negative result with a DNA probe for M. avium complex(Accuprobe; GenProbe) eliminated this hypothesis. In comparisonto other slowly growing strains of mycobacteria, this isolatecould be distinguished from M. genavense by its ability to growon standard mycobacterial solid media (2). The lack of ureaseand the yellow pigmentation eliminated M. simiae (12), M. malmoense(12), and M. triplex (6).

Because of a lack of results by conventional testing, different nucleic acid analyses were performed with the DNA of the HL1clinical strain. They included PCR-restriction enzyme patternanalysis (PRA) of the hsp65 gene (1), PCR amplification, andsequencing analysis of the 16S rRNA gene (9) and of the 16S-23SrRNA gene internal transcribed spacer region (ITS) (11). Thesequences obtained were compared to known 16S rRNA and ITS sequencesavailable in GenBank by pairwise and multiple-sequence alignmentswith LALIGN (Infobiogen), CLUSTALW (Infobiogen), and BLAST (NationalCenter for Biotechnology Information)software.

The PRA pattern, based on the results obtained by digestion with both BstEII and HaeIII enzymes, showed two fragments of 150and 135 bp with HaeIII but no restriction site with BstEII. Thispattern was compatible with the PRA results previously describedfor M. lentiflavum and differed from those described for M. simiae(12), M. genavense (12), and M. malmoense (1). The 482-bp16S rRNA fragment sequenced from isolate HL1 showed 100% identitywith the sequence of the M. lentiflavum reference strain (12).Homologies with the 16S rRNA sequences of M. simiae (10) andM. triplex (6), M. genavense (2), and M. malmoense (10)were lower, with 98, 97, and 93.7% identities,respectively.

In the sequence comparison with the BLAST software, the best homologies found for the 283-bp ITS PCR fragment of isolate HL1were with the ITS sequences of M. triplex (11), M. genavense(11), and M. simiae (8). It should be noted that the 16S-23SrRNA gene ITS sequence of M. lentiflavum was not available inthe sequence libraries. Therefore, we amplified and sequenceda 413-bp PCR fragment encompassing the 131-bp 3' end of the 16SrRNA gene and the 282-bp complete ITS sequence of the referencestrain of M. lentiflavum (ATCC 51985). Like other slow growers(11), M. lentiflavum showed a short ITS sequence of 282 bp.This sequence was found to be closely related to the ITS sequencesof the mycobacterial cluster comprising M. triplex (92.3% identity),M. genavense (90.8% identity), and M. simiae (90.1% identity).These homology data are in good agreement with those obtainedfor 16S rRNA (6, 11, 12), which found M. lentiflavum tobe closely related to M. simiae, M. triplex, and M. genavense.

The comparison of the ITS sequence of the HL1 isolate with those of M. lentiflavum (this study), M. triplex (11), M. genavense(11), and M. simiae (8) showed 21 base differences (92.6%identity), 13 differences (95.4% identity), 14 differences (95.1%identity) and 25 differences (91.2% identity), respectively. Figure1 shows the alignments of the ITS sequences from the HL1 isolateand M. lentiflavum, M. simiae, M. triplex, and M. genavense. TheITS sequence analysis gave an identification different from thatprovided by 16S rRNA sequencing and incompatible with the phenotypiccharacteristics of isolate HL1. On the basis of the phenotypicand genotypic data, we identified isolate HL1 as an M. lentiflavumstrain.

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FIG. 1. Alignment of complete 16S-23S rRNA ITS sequences from isolate HL1 (HL1), M. lentiflavum ATCC 51985 (ML), M. simiae (MS; GenBank accession no. AB026694), M. triplex (MT; GenBank accession no. Y14189), and M. genavense (MG; GenBank accession no. Y14183). The lengths of the ITS sequences (in nucleotides) are indicated at the end of the sequences. The complete ITS sequence between the end of the 16S rRNA gene and the beginning of the 23S rRNA gene is shown. Dashes indicate aligment gaps, and asterisks indicate variable nucleotide positions.

Discussion. Disease caused by nontuberculous mycobacteria (NTM) is common among patients with AIDS. The most common species isolated isthe M. avium complex, although the other species including thegroup of slowly growing NTM such as M. genavense, M. malmoense,M. simiae, and M. triplex have also been described as causes ofdisseminated disease (3, 5). We report here on the firstcase of a disseminated infection in an HIV-infected patient causedby M. lentiflavum, a species recently described by Springer etal. (12). Among the 22 isolates reported by Springer et al.(12), most were isolated fortuitously or were traced to contaminatedbronchoscopes. Only one isolate was recovered from a patient withspondylodiscitis (12), and another isolate was recovered froma patient with cervical lymphadenitis (7).

The pattern of results obtained by conventional identification procedures, including colony, biochemical, and enzymatic tests,failed to match the patterns of any reported mycobacterial species.The identification of this isolate was accomplished by 16S rRNAsequencing and was confirmed by PCR-PRA of the hsp65 gene. Inthe present study we also compared the rRNA ITS sequence of thisisolate (HL1) with that of the M. lentiflavum reference strain(ATCC 51985). Comparison of the ITS sequences provides guidanceon the possible divergence of the ITS sequence within this relativelynew species. In summary, we report the first case of disseminatedM. lentiflavum infection in an AIDS patient documented by both16S rRNA gene sequencing and PCR-PRA of the hsp65gene.

Nucleotide sequence accession numbers. The ITS gene sequences of the M. lentiflavum reference strain (ATCC 51985) and of the HL1 clinical isolate were submittedto GenBank and given accession no. AF317658 and accession no.AF318174,respectively.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire de Bactériologie, Université Victor Segalen Bordeaux 2, 146 rue LéoSaignat, 33076 Bordeaux cedex, France. Phone: (33) 5.57.57.16.25.Fax: (33) 5.56.93.29.40. E-mail: jeannette.maugein{at}ubordeaux2.fr.

REFERENCES

Top
Abstract
Case Report
References

1. Devallois, A., K. Seng Goh, and N. Rastogi. 1997. Rapid identification of mycobacteria to species level by PCR restriction fragment length polymorphism analysis of the hsp65 gene and proposition of an algorithm to differentiate 34 mycobacterial species. J. Clin. Microbiol. 35:2969-2973[Abstract].

2. Böttger, E. C., B. Hirschel, and M. B. Coyle. 1993. Mycobacterium genavense sp. nov. Int. J. Syst. Bacteriol. 43:841-843[Abstract/Free Full Text].

3. Cingolani, C., M. Sanguinetti, A. Antinori, L. M. Larocca, F. Ardito, B. Posteraro, G. Federico, G. Fadda, and L. Ortona. 2000. Disseminated mycobacteriosis caused by drug-resistant Mycobacterium triplex in a human immunodeficiency virus-infected patient during highly active antiretroviral therapy. Clin. Infect. Dis. 31:177-179[CrossRef][Medline].

4. David, H., V. Lévy-Frébault, and M. F. Thorel. 1989. Methodes de laboratoire pour mycobactériologie clinique. Commission des Laboratoires d'Expertise et de Référence, Institut Pasteur, Paris, France.

5. Falkinham, J. 1996. Epidemiology of infection by nontuberculous mycobacteria. Clin. Microbiol. Rev. 9:177-215[Medline].

6. Floyd, M., L. S. Guthertz, V. A. Silcox, P. S. Duffey, Y. Jang, E. P. Desmond, J. T. Crawford, and W. R. Butler. 1996. Characterization of an SAV organism and proposal of Mycobacterium triplex sp. nov. J. Clin. Microbiol. 34:2963-2967[Abstract].

7. Haase, G., H. Kentrup, H. Skopnic, B. Springer, and E. C. Böttger. 1997. Mycobacterium lentiflavum: an etiologic agent of cervical lymphadenitis. Clin. Infect. Dis. 25:1245-1246[Medline].

8. Kasai, H., T. Ezaki, and S. Harayama. 2000. Differentiation of phylogenetically related slowly growing mycobacteria by their gyrB sequences. J. Clin. Microbiol. 38:301-308[Abstract/Free Full Text].

9. Kirschner, P., B. Springer, U. Vogel, A. Meier, A. Wrede, M. Kiekenbeck, F. C. Bange, and E. C. Böttger. 1993. Genotypic identification of mycobacteria by nucleic acid sequence determination: report of a 2-year experience in a clinical laboratory. J. Clin. Microbiol. 31:2882-2889[Abstract/Free Full Text].

10. Rogall, T., J. Wolters, T. Flohr, and E. C. Böttger. 1990. Towards a phylogeny and definition of species at the molecular level within the genus Mycobacterium. Int. J. Syst. Bacteriol. 40:323-330[Abstract/Free Full Text].

11. Roth, A., M. Fischer, M. E. Hamid, S. Michalke, W. Ludwig, and H. Mauch. 1998. Differentiation of phylogenetically related slowly growing mycobacteria based on 16S-23S rRNA gene internal transcribed spacer sequences. J. Clin. Microbiol. 36:139-147[Abstract/Free Full Text].

12. Springer, B., W. Wu, T. Bodmer, G. Haase, G. E. Pfyffer, R. M. Kroppenstedt, K. H. Schröder, S. Emler, J. O. Kilburn, P. Kirschner, A. Telenti, M. B. Coyle, and E. C. Böttger. 1996. Isolation and characterization of a unique group of slowly growing mycobacteria: description of Mycobacterium lentiflavum sp. nov. J. Clin. Microbiol. 34:1100-1107[Abstract].

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1.	Devallois, A., K. Seng Goh, and N. Rastogi. 1997. Rapid identification of mycobacteria to species level by PCR restriction fragment length polymorphism analysis of the hsp65 gene and proposition of an algorithm to differentiate 34 mycobacterial species. J. Clin. Microbiol. 35:2969-2973[Abstract].
2.	Böttger, E. C., B. Hirschel, and M. B. Coyle. 1993. Mycobacterium genavense sp. nov. Int. J. Syst. Bacteriol. 43:841-843[Abstract/Free Full Text].
3.	Cingolani, C., M. Sanguinetti, A. Antinori, L. M. Larocca, F. Ardito, B. Posteraro, G. Federico, G. Fadda, and L. Ortona. 2000. Disseminated mycobacteriosis caused by drug-resistant Mycobacterium triplex in a human immunodeficiency virus-infected patient during highly active antiretroviral therapy. Clin. Infect. Dis. 31:177-179[CrossRef][Medline].
4.	David, H., V. Lévy-Frébault, and M. F. Thorel. 1989. Methodes de laboratoire pour mycobactériologie clinique. Commission des Laboratoires d'Expertise et de Référence, Institut Pasteur, Paris, France.
5.	Falkinham, J. 1996. Epidemiology of infection by nontuberculous mycobacteria. Clin. Microbiol. Rev. 9:177-215[Medline].
6.	Floyd, M., L. S. Guthertz, V. A. Silcox, P. S. Duffey, Y. Jang, E. P. Desmond, J. T. Crawford, and W. R. Butler. 1996. Characterization of an SAV organism and proposal of Mycobacterium triplex sp. nov. J. Clin. Microbiol. 34:2963-2967[Abstract].
7.	Haase, G., H. Kentrup, H. Skopnic, B. Springer, and E. C. Böttger. 1997. Mycobacterium lentiflavum: an etiologic agent of cervical lymphadenitis. Clin. Infect. Dis. 25:1245-1246[Medline].
8.	Kasai, H., T. Ezaki, and S. Harayama. 2000. Differentiation of phylogenetically related slowly growing mycobacteria by their gyrB sequences. J. Clin. Microbiol. 38:301-308[Abstract/Free Full Text].
9.	Kirschner, P., B. Springer, U. Vogel, A. Meier, A. Wrede, M. Kiekenbeck, F. C. Bange, and E. C. Böttger. 1993. Genotypic identification of mycobacteria by nucleic acid sequence determination: report of a 2-year experience in a clinical laboratory. J. Clin. Microbiol. 31:2882-2889[Abstract/Free Full Text].
10.	Rogall, T., J. Wolters, T. Flohr, and E. C. Böttger. 1990. Towards a phylogeny and definition of species at the molecular level within the genus Mycobacterium. Int. J. Syst. Bacteriol. 40:323-330[Abstract/Free Full Text].
11.	Roth, A., M. Fischer, M. E. Hamid, S. Michalke, W. Ludwig, and H. Mauch. 1998. Differentiation of phylogenetically related slowly growing mycobacteria based on 16S-23S rRNA gene internal transcribed spacer sequences. J. Clin. Microbiol. 36:139-147[Abstract/Free Full Text].
12.	Springer, B., W. Wu, T. Bodmer, G. Haase, G. E. Pfyffer, R. M. Kroppenstedt, K. H. Schröder, S. Emler, J. O. Kilburn, P. Kirschner, A. Telenti, M. B. Coyle, and E. C. Böttger. 1996. Isolation and characterization of a unique group of slowly growing mycobacteria: description of Mycobacterium lentiflavum sp. nov. J. Clin. Microbiol. 34:1100-1107[Abstract].