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Journal of Clinical Microbiology, July 2002, p. 2668-2670, Vol. 40, No. 7
0095-1137/02/$04.00+0 DOI: 10.1128/JCM.40.7.2668-2670.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.
Departments of Ophthalmology,1 Microbiology, University Hospital,2 Department of Laboratory Medicine, Norwegian University of Science and Technology, N-7006 Trondheim, Norway3
Received 26 November 2001/ Returned for modification 3 February 2002/ Accepted 7 April 2002
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Staphylococci, in particular Staphylococcus epidermidis, are most frequently involved in infections in the early postoperative period (4, 13), whereas streptococci, in particular the viridans group, are most frequently found in late-onset endophthalmitis, in addition to Haemophilus influenzae and a variety of other bacteria (4, 8, 12).
Moraxella spp. are a group of gram-negative, oxidase- and catalase-positive coccobacilli, often found as commensals in the upper respiratory tract and considered to have low pathogenic potential. Here we report two cases of late-onset posttrabeculectomy endophthalmitis caused by Moraxella nonliquefaciens.
Case 1. A 78-year-old man was admitted on 2 September 1999 with a 1-day history of purulent discharge and 12 h of decreased visual acuity in his right eye. In 1990 he had undergone trabeculectomy, and in 1994 cataract surgery had been performed. On admission visual acuity was light perception, intraocular pressure was 32 mm Hg, the bulb was hyperemic, and the cornea was edematous. The filtering bleb was pale, and a grade III reaction in the anterior chamber and vitreous clouding were observed. No red reflex was seen. Vitreous and anterior chamber taps were performed. Vancomycin (100 µg) and gentamicin (100 µg) were administered intravitreally, and cefuroxime (200 µg) was instilled into the anterior chamber. The patient received intravenous gentamicin (80 mg every 8 h) and vancomycin (500 mg every 12 h) as well as oral prednisolone. Cefuroxime and gentamicin eyedrops were administered topically. Altogether, the patient received three intravitreal injections of vancomycin and gentamicin. On one occasion, bleeding in the anterior chamber occurred, probably due to an increased bleeding tendency, as he was receiving warfarin prophylaxis against cerebral thromboembolism. A pupillary membrane developed, and he never regained a visual acuity of more than light perception. Culture of the anterior chamber fluid grew gram-negative coccobacillary organisms (strain 96127/99), but culture from the vitreous humor and the conjunctiva yielded no growth.
Case 2. A 76-year-old man was admitted on 20 December 2000 with a history of acute blurred vision of his right eye of a few hours' duration. On the day prior to admission, he had observed purulent discharge. Cataract surgery had been performed in 1996. Two months prior to the actual episode, he had undergone a trabeculectomy with instillation of mitomycin C subconjunctivally. The visual acuity of his right eye was hand motions, and the intraocular pressure was 13 mm Hg. A diffuse edema of the palpebra was noted, mucus was present in the cilia, and the cornea appeared edematous. The filtering bleb was broadbased, heavily injected except at the 2 o'clock position, where it was pale, thin, and probably distended with pus. The reaction in the anterior chamber was heavy with clouding and fibrinous exudates. No red reflex was observed, and the fundus could not be visualized. An ultrasound scan, however, demonstrated dense clouding of the vitreous humor, in particular inferiorly and temporally. Vitreous and anterior chamber taps were performed, vancomycin (100 µg) and gentamicin (100 µg) were administered intravitreally, and cefuroxime (200 µg) was instilled into the anterior chamber. This procedure was repeated once 2 days later. The patient also received topical treatment with gentamicin and cefuroxime eyedrops, as well as oral prednisolone. He was discharged after 13 days. The visual acuity was only light perception, and after 6 months it was no better than hand motions. A Gram stain of the vitreous humor collected on admission demonstrated numerous polymorphonuclear leukocytes and gram-variable, mainly gram-negative, small rods. Culture from the anterior chamber and the conjunctiva yielded no growth, but in culture from the vitreous humor there was abundant growth of a gram-negative coccobacillary organism (strain 141365/00).
Microbiology. In both cases the specimens were immediately transported to the laboratory and processed within 6 h after being taken.
A phenotypic characterization of the two M. nonliquefaciens strains is given in Table 1. By using API NH (bioMerieux, Marcy l'Étoile, France) both strains generated profile 0010, interpreted by the database (version 2.0) as excellent identification of Moraxella (subgen. Branhamella) catarrhalis (percent identity, 99.9%; T index value = 1.00) but suggesting the possibility of other Moraxella spp. DNase positivity has been used as a main phenotypic characteristic for distinguishing M. catarrahalis from other Moraxella spp. (3). After 48 h of growth, the DNase test agar (Difco) was flooded with 1 M HCl. A narrow zone of incomplete clearing around the growth was observed for one of the isolates (Table 1), while M. catarrhalis produced a wide zone of complete clearing of the agar.
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TABLE 1. Phenotypic characteristics of two M. nonliquefaciens strains
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TABLE 2. Antibiotic susceptibilities of two M. nonliquefaciens strains
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The microscopic morphology and growth characteristics of the two strains closely resemble the description of M. nonliquefaciens (2). Identification of Moraxella spp. other than M. catarrhalis is not always straightforward. The microscopic morphology (coccobacilli, not diplococci) and soft, glistening colonies (as opposed to dry colonies that can be swept intact over the agar surface) are atypical for M. catarrhalis, the species suggested by the API NH database. To our knowledge, weak DNase activity, as observed for one of the present strains, has not been reported for M. nonliquefaciens. By combining phenotypic characteristics and 16S rRNA gene sequencing, we consider the identification of both strains as M. nonliquefaciens to be reliable. The main natural habitat of M. nonliquefaciens is most probably the human nasal cavity, and this organism has mostly been isolated from respiratory and ocular sites (6).
We are aware of only six published cases of endophthalmitis caused by M. nonliquefaciens. The first report, by Ebright in 1981, concerned an immunocompromised patient believed to have contracted the infection through minor trauma of the cornea from a contact lens (5). For the other five patients, trabeculectomy had been performed, with an interval from surgery to endophthalmitis ranging from 2 months to 15 years (11, 12, 15, 16). Our two cases of late-onset endophthalmitis caused by M. nonliquefaciens after glaucoma filtering surgery clearly demonstrate the devastating outcome of this infection, even though the causative organism is generally considered to be of low virulence and the antibiotics given are considered adequate. In both cases the course was very rapid, with acute onset of decreased vision. Both patients had noted a purulent discharge from the conjunctiva within the 24 h prior to onset of endophthalmitis. For our two patients, M. nonliquefaciens was not detected in conjunctival cultures. A poor correlation between conjunctival cultures and intraocular cultures has been observed previously. Of 18 patients for whom conjunctival and intraocular cultures yielded microorganisms, only 5 had the same bacterium cultured from the conjunctiva and the aqueous or vitreous humor (12), whereas in another study 4 of 16 cases showed concordance between conjunctival and intraocular cultures (4). It is reasonable, therefore, to infer that organisms entering intraocularly through the filtering bleb may be present only transiently on the bleb surface. It is also important to realize that conjunctival cultures in this setting may be misleading. Awareness of the risk of endophthalmitis in patients who have undergone filtering-bleb surgery is necessary.
Nucleotide sequence accession numbers. The nucleotide sequences of the 16S rRNA genes of strains 96127/99 and 141365/00 have been given GenBank accession numbers AF443790 and AF443789, respectively.
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