Emerging Infectious Diseases
[Volume 5 No.1 / January - February 1999]

Suggested Citation

Dispatches

Mycoplasma penetrans Bacteremia and Primary Antiphospholipid Syndrome(ft 1)

(ft 1)Presented in part at the 11th International Congress of the International
Organization for Mycoplasmology. July 14–19, 1996. Orlando, FL, USA.

Antonio Yáñez,* Lilia Cedillo,† Olivier Neyrolles,‡ Encarnación Alonso,*
Marie-Christine Prévost,‡ Jorge Rojas,* Harold L. Watson,§ Alain
Blanchard,‡ and Gail H. Cassell§
*Centro de Investigación Biomédica de Oriente-IMSS, Puebla City, Mexico;
†Benemérita Universidad Autónoma de Puebla, Puebla City, Mexico; ‡Institut
Pasteur, Paris, France; and §University of Alabama at Birmingham,
Birmingham, Alabama, USA

---------------------------------------------------------------------------
      Mycoplasma penetrans, a rare bacterium so far only found in
      HIV-infected persons, was isolated in the blood and throat of a
      non-HIV-infected patient with primary antiphospholipid syndrome
      (whose etiology and pathogenesis are unknown).

Antiphospholipid syndrome (APS), first described in 1983 to 1986, is
characterized by a wide variety of hemocytopenic and vaso-occlusive
manifestations and is associated with antibodies directed against
negatively charged phospholipids. Features of APS include hemolytic anemia,
thrombocytopenia, venous and arterial occlusions, livedo reticularis,
pulmonary manifestations, recurrent fetal loss, neurologic manifestations
(stroke, transverse myelitis, Guillain-Barré syndrome); and a positive
Coombs test, anticardiolipin antibodies, or lupus anticoagulant activity
(1). The factor(s) causing production of the antiphospholipid antibodies in
primary antiphospholipid syndrome (PAPS) remain unidentified (2).

A substantial number of patients with Mycoplasma pneumoniae–induced
respiratory disease have anticardiolipin antibodies (3). Furthermore, many
clinical criteria for APS have also been well documented in patients with
M. pneumoniae infection, including Guillain-Barré–like illness and other
central nervous system manifestations, hemolytic anemia, positive Coombs
test, thrombocytopenia, and arthritis (4).

In this report, we describe the case of a patient with clinical features of
PAPS and a documented bacteremic infection due to M. penetrans (5).

Case

One month before hospital admission, a previously healthy non-HIV-infected
17-year-old woman (blood group O Rh+) who had not previously received a
blood transfusion and had not had sexual experience had acute onset of
arthritis of both ankles, generalized arthralgias, fever, progressive
asthenia, and hemolytic anemia (hemoglobin 87 g/L, unconjugated bilirubin
25.1 µmol/L). In the 30 days before hospital admission she had not received
medications other than nonsteroidal antiinflammatory drugs for 5 days.
Three days before hospital admission, she became ill with respiratory
distress, generalized weakness, anorexia, and inability to walk.

On admission to the hospital (day 1), physical examination showed severe
pallor, a swollen cervical lymph node, slight edema of both legs,
tachycardia, and no hypertension. Laboratory data showed severe hemolytic
anemia (hemoglobin 34 g/L, lactate dehydrogenase 5.1 µmol/s/L),
leukocytosis (24.5 x 10[sup 9]/L), thrombocytopenia (28.0 x 10[sup 9]/L), and normal
renal function. A Coombs test was positive at 4ºC, 22ºC, and 37ºC. Blood
and bone marrow smears did not show a neoplasic process. The nonsteroidal
antiinflammatory drugs were suspended, and treatment was started with a
combination of methylprednisolone (1 gm bolus q24h intravenously [i.v.] for
3 days) and trimethoprim/sulfamethoxazole (80/400 mg q12h orally) on day 2,
but her condition deteriorated. On day 3, the antibiotic treatment was
changed to ceftazidime (1 gm q8h i.v.). Transfusion was not attempted
because serologic tests indicated the lack of compatibility; (there was a
strong positive mismatch incompatibility in 55 different blood samples and
a mild mismatch in one sample). Another transfusion was partially rejected
because of unidentified nonspecific antibodies. On day 4 severe respiratory
distress and hypoxemia developed, requiring a ventilator, and the patient
was admitted to the intensive care unit. Livedo reticularis was noted, and
methylprednisolone (125 mg q8h i.v.) was administered. Venereal Disease
Research Laboratory tests were negative as were tests for lupus
erythematosus. The patient had anti-dsDNA antibodies (Kallestad Quantafluor
Crithidia lucilae Sanofi Diagnostic Pasteur, Inc.) but positive
anticardiolipin antibodies by enzyme-linked immunosorbent assay (ELISA)
(100 GPL units) (negative test = <10 GPL units) (ImmunoWell, Cardiolipin
Antibody Immunoglobulin [Ig]G ELISA; and Reaads Medical Products, Inc.),
which remained positive 4 and 12 months later, and antiplatelet antibodies
by immunofluorescence (Anti-Human IgG H-chain Fluorescein conjugated,
OTIY-05 Behring Diagnostics). Laboratory data showed hemoglobin 33 g/L,
leukocyte 23.6 x 10[sup 9]/L, a prolonged activated partial thromboplastin time
>150 seconds (control <42 seconds) and prothrombin time of 26.1 seconds
(control 14.0 seconds), International Normalized Ratios value = 3D 2.09,
and the presence of lupus anticoagulant (LA) antibodies (prolonged Russell
viper venom time and confirmed by the STACLOT LA ELISA test, Reaads Medical
Products, Inc.). Respiratory secretions were culture-negative and negative
by immunofluorescence for respiratory syncytial virus, adenovirus,
influenza A, influenza B, parainfluenza 1,2,3, and Chlamydia. Serologic
analysis indicated that the patient had no antibodies against HIV,
hepatitis B surface and core antigens (HbsAg, HBc), or hepatitis C virus.
No acid-fast bacilli or other bacteria were observed on blood and tracheal
aspirate smears. In addition, thoracic radiography showed only bilateral
diffuse pulmonary infiltrates, which was not suggestive of an anaerobic
infection.

On day 2 of hospital admission, blood and throat samples were cultured for
aerobic flora and mycoplasma. M. penetrans in pure culture was isolated
from the patient's blood (isolate HF-1) and throat (isolate HF-3). Later M.
penetrans was isolated from tracheal aspirate in pure culture (isolate
HF-2). Treatment was initiated on day 6 with clindamycin 600 mg q8h i.v.
and vancomycin 500 mg q6h i.v. The patient also received transfusion of two
units of washed red blood cells.

By the microbroth dilution method (6), the HF-1 isolate was sensitive to
clindamycin, clarithromycin, azithromycin, erythromycin, tetracycline,
doxycycline, ofloxacin, and chloramphenicol but resistant to vancomycin and
gentamicin. After 3 days of treatment, the patient improved clinically and
was released from the intensive care unit on day 9; thoracic radiographs
were clear.

The unique evidence of thrombosis was a low-degree paresthesia of both legs
while the patient was receiving anticoagulant therapy; when the condition
developed, anticoagulant therapy was increased. The patient received
physiotherapy to correct paresis and reduced sensation in the left foot and
ankle region. She left the hospital after 26 days, with minimal evidence of
peripheral neuropathy as a sequela.

M. penetrans infection was detected in the patient's specimens prior to
culture and was confirmed by specific polymerase chain reaction (PCR) (7)
(Figure 1A, 1B). Similar results were obtained by another pair of PCR
primers also within the 16S rRNA gene and designed for the specific
detection of M. penetrans (data not shown). Samples from both original
specimens and broth cultures were tested by PCR for other human mycoplasmas
(8,9), but none were detected (data not shown).


[Fig] 
Figure 1. Polymerase chain reaction (PCR)
detection of Mycoplasma penetrans in clinical samples. A. M. penetrans 
PCR genomic amplification with the primers MYCPENET-P and MYCPENET-N (7) 
and analyzed by electrophoresis in 2% agarose gel. Lysates from the 
following original samples: throat swab (lane 1); tracheal aspirate 
(lane 2); blood (lane 3); first blood subculture (HF-1 isolate) (lane 4); 
M. penetrans GTU-54-6A1 (lane 5), showing the amplification product of 
407-bp; and negative control (lane 6). B. Southern blotting of the same 
material. Hybridization with the internal oligonucleotide (MYCPENET-S) probe 
confirmed the specific amplification of M. penetrans genetic sequences.

The sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)
protein patterns of different extracts (whole cell lysate, Triton X-114
extracts) for the isolate HF-1 and the type strain GTU-54-6A1 were almost
identical (Figure 2A). Upon close examination, minor differences were
found, in particular for antigens approximately 38 kDa in both SDS and
Triton X-114 extracts. Ultrastructural examination of the HF isolates by
transmission electron microscopy showed mycoplasma cells with morphologic
features typical of M. penetrans (Figure 2B).


[Fig]
Figure 2. HF isolates belong to the species Mycoplasma penetrans. A. 
Comparison of protein patterns from the type strain of M. penetrans and the 
isolate HF-1. Mycoplasma cells were directly lysed with SDS (cell lysate), 
or antigens were extracted with the neutral detergent Triton X-114 (total
extract). Antigens were further separated after partitioning between the 
aqueous and detergent phases. The two mycoplasmas compared are the M. 
penetrans type strain GTU-54-6A1 (GTU) and the isolate HF. B. Ultrastructural 
features of the M. penetrans isolates HF-1, HF-2 and HF-3. The HF isolates
were passaged four times in SP-4 broth without antibiotics and processed for
transmission electron microscopy (TEM). Ultrathin sections were stained 
with osmiun tetroxide and ruthenium red and observed by TEM. The three 
isolates show the typical elongated, flask-shaped morphology of M.
penetrans, with the two divided internal compartments. The cytoplasm is 
limited by a single triple-layered unit membrane that is covered with 
capsular material.

Serologic assays (ELISA and Western blot) with Triton X-114-extracted
antigens and other M. penetrans polypeptides from whole-cell lysates both
from the type strain GTU-54-6A1 and from our isolate HF-1 were done as
previously described (10). A lack of reactivity against the Triton
X-114–extracted antigens of M. penetrans was observed by both methods.
However, with whole-cell extracts from both type strain and the HF-1
isolate, a 20-kDa polypeptide was immunodetected by Western blotting with
three serum samples collected on days 2, 4, and 9 of hospitalization. The
20-kDa polypeptide is an M. penetrans product, but whether the observed
reaction corresponds to a cross-reacting epitope is not known. The
patient's samples were also negative for antibodies against M. pneumoniae,
M. genitalium, and M. fermentans by ELISA (11) (data not shown).

Conclusions

Since M. penetrans was first reported in 1993 as an emerging infectious
agent, M. penetrans–specific antibodies have been detected more frequently
(18.2% to 35.4%) in HIV-infected than in non-HIV-infected persons (0.4% to
1.3%) (10). Until this case, M. penetrans had only been isolated eight
times (5,10), always from the urine of HIV-infected persons (10).

The results indicating that the isolates HF-1, HF-2, and HF-3 belong to the
M. penetrans species are as follows: 1) clinical samples and the
mycoplasmal isolates obtained from them were positive in the M.
penetrans-specific PCR assay; 2) protein patterns of the HF isolates and
the type strain of M. penetrans GTU-54-6A1 were almost identical; 3) serum
samples from different patients (10), which contained M. penetrans-specific
antibodies on the basis of a reaction with the p35 antigen from the type
strain of M. penetrans also reacted with a similar Triton X-114–extracted
polypeptide from the HF-1 isolate; and 4) HF isolates exhibited typical
morphologic features of M. penetrans, which are unique among mycoplasmas
isolated from humans. The fact that serum from other patients reacted with
a similar polypeptide from HF isolates indicates that this protein is
produced by this strain of M. penetrans. The lack of M. penetrans strong
humoral response in the HF patient was a factor in favor of dissemination
of the mycoplasma, hence its isolation from the blood. A possible
association between M. penetrans and PAPS should be considered.

Snowden et al. (1990) found antiphospholipid antibodies in more than 50% of
patients with M. pneumoniae pneumonia, especially those with severe
infections requiring hospitalization (3). Catteau et al. (1995) described
two cases of Stevens-Johnson syndrome associated with M. pneumoniae
infection and the presence of antiphospholipid antibodies (12). Our patient
had manifestations typical of PAPS (2). Thus, this report is the first of
M. penetrans isolation in a non-HIV-infected patient and the first of a
blood and respiratory tract infection with M. penetrans.

Acknowledgments

      The authors thank Constantino Gil, M. Ran Nir-Paz, Donna C. Crabb,
Lynn B. Duffy, Padma Patel, Blanca Tobón, Angeles Ríos, and Eduardo Aguirre
for technical contributions.

      This work was supported in part by grant R01 AR 42469, National
Institute of Arthritis and Metabolism, National Institutes of Health; the
Institut Pasteur; and FOSIZACONACYT grant 960202008.

      Dr. Yáñez is researcher in the Eastern Biomedical Research Center
(Centro de Investigación Biomédica de Oriente), IMSS. He has worked with
human mycoplasmas for the last 12 years and is interested in bacterial
pathogenesis, in particular in the field of autoimmune diseases triggered
by mycoplasmas.

      Address for correspondence: Antonio Yáñez, Centro de Investigación
Biomédica de Oriente-IMSS, 2º Piso Ala Sur, Hospital de Especialidades, 2
Norte 2004, 72000 Puebla City, Mexico; fax: 52-22-46-00-57; e-mail:
ayanez@gemtel.com.mx.

References

  1. Hughes GRV. The antiphospholipid syndrome: ten years on. Lancet
     1993;342:341-4.
  2. Asherson RA, Cervera R. "Primary," "secondary," and other variants of
     the antiphospholipid syndrome. Lupus 1994;3:293-8.
  3. Snowden N, Wilson PB, Longson M, Pumphrey RSH. Antiphospholipid
     antibodies and Mycoplasma pneumoniae infection. Postgrad Med J
     1990;66:356-62.
  4. Cassell GH, Gray G, Waites KB. Chapter 180: mycoplasmal infections.
     In: Harrison's principles of internal medicine. Isselbacher KJ,
     Braunwald E, Wilson JD, Martin JB, Fauci AS, Kasper DL, editors. Vol.
     1, McGraw-Hill Inc, 1997:1052-55.
  5. Lo S-C, Hayes MM, Tully JG, Wang RY-H, Kotani H, Pierce PF, et al.
     Mycoplasma penetrans sp. nov., from the urogenital tract of patients
     with AIDS. Int J Syst Bacteriol 1992;42:357-64.
  6. Waites KB, Cassell GH, Cannupp KC, Fernandes PB. In vitro
     susceptibilities of mycoplasmas and ureaplasmas to new macrolides and
     aryl-fluoroquinolones. Antimicrob Agents Chemother 1988;32:1500-2.
  7. Grau O, Kovacic R, Griffais R, Launay V, Montagnier L. Development of
     a PCR-based assays for the detection of two human mollicute species,
     Mycoplasma penetrans and M. hominis. Mol Cell Probes 1994;8:139-48.
  8. Blanchard A, Gautier M, Mayau V. Detection and identification of
     mycoplasmas by amplification of rDNA. FEMS Microbiol Lett
     1991;81:37-42.
  9. Blanchard A, Yáñez A, Watson H, Griffiths G, Cassell GH. Evaluation of
     intraspecies genetic variation within the 16S rRNA gene of Mycoplasma
     hominis and detection by polymerase chain reaction. J Clin Microbiol
     1993;31:1358-61.
 10. Grau O, Slizewicz B, Tuppin P, Launay V, Bourgeois E, Sagot N, et al.
     Association of Mycoplasma penetrans with immunodeficiency virus
     infection. J Infect Dis 1995;172:672-81.
 11. Cassell GH, Gambil G, Duffy LB. ELISA in respiratory infections of
     humans. In: Molecular and diagnostic procedures in mycoplasmology. Vol
     II. Tully JG, Razin S, editors. Academic Press 1996:123-36.
 12. Catteau B, Delaporte E, Hachulla E, Piette F, Bergoend H. Infection à
     mycoplasme avec syndrome de Stevens-Johnson et anticorps
     antiphospholipides: à propos de deux cas. Rev Med Interne
     1995;16:10-4.

Emerging Infectious Diseases
National Center for Infectious Diseases
Centers for Disease Control and Prevention
Atlanta, GA

URL: ftp://ftp.cdc.gov/pub/EID/vol5no1/ascii/yanez.txt

Please note that figures and equations are not available in ASCII format; 
their placement within the text is noted by [fig] and [eq], respectively. 
Greek symbols are spelled out. The following codes are used: 
(ft) for footnote; (sup) for superscript; (sub) for subscript; 
>/= for greater than or equal to.