1.A Case of Cryptococcosis involving Lung and CNS without Underlying Disease.
Min Su LEE ; Sang Seon PARK ; Young Il KOH ; An Soo JANG ; Sung Chul LIM ; Ju Yeoul YANG ; Hyung Kwan PARK ; Hyun Joo NA ; Young Chul KIM ; In Seon CHOI ; Kyung Ok PARK
Tuberculosis and Respiratory Diseases 1995;42(4):618-623
Cryptococcosis is a systemic mycosis that most often involves the lungs and central nervous system and, less frequently, the skin, skeletal system, and prostate gland. Cryptococcus neoformans, the causative organism, is a yeastlike round or oval fungus, 4 to 6microm in diameter, which is surrounded by a polysaccharide capsule and reproduces by budding and found in soil and other enviromental areas, especially those contaminated by pigeon droppings. Humans and aninmals acquire infection after inhalation of aerosolized spores. Condition or factors that predispose to cryptococcosis include corticosteroid therapy, lymphoreticular malignancies, HIV infection, and sarcoidosis etc. We discribed a case of cryptococcosis involving lung and CNS coincidently without specific underlying disease and the literature on subject were reviewed. A fifty-six year-old previously healthy female presented with headache of 3 months of duration. She had no history suggesting immunologic suppression and we could not find any abnormal laboratory findings including blood sugar, serum immunoglobulin and complement level, HIV antibody, and T cell subsets. Chest roentgenogram and CT scan showed a solitary soft tissue mass in LUL with distal pneumonitis. Brain MRI showed granulomatous lesion in cerebellum and parasagittal cortex of right frontal lobe. The diagnosis was made by bronchoscopic brushing cytology, transthoracic fine needle aspiration, and sputum OH mount and culture. She was treated 6 weeks course of Amphotericin B and switched to oral fluconazole therapy for 3 months. Her symptoms and X-ray findings were improved gradually and she is now under regular clinical follow up.
Amphotericin B
;
Biopsy, Fine-Needle
;
Blood Glucose
;
Brain
;
Central Nervous System
;
Cerebellum
;
Columbidae
;
Complement System Proteins
;
Cryptococcosis*
;
Cryptococcus neoformans
;
Diagnosis
;
Female
;
Fluconazole
;
Follow-Up Studies
;
Frontal Lobe
;
Fungi
;
Headache
;
HIV
;
HIV Infections
;
Humans
;
Immunoglobulins
;
Inhalation
;
Lung*
;
Magnetic Resonance Imaging
;
Pneumonia
;
Prostate
;
Sarcoidosis
;
Skin
;
Soil
;
Spores
;
Sputum
;
T-Lymphocyte Subsets
;
Thorax
;
Tomography, X-Ray Computed
2.DNA Fingerprinting of Candida albicans Strains Isolated from Candidemic Patients by Polymerase Chain Reaction and Southern Hybridization Methods.
Ju Yeoul PARK ; Jong Hee SHIN ; Sung Jin YANG ; Bong Joon OH ; Duck CHO ; Seong Jung KEE ; Myung Gun SHIN ; Soon Pal SUH ; Dong Wook RYANG
Infection and Chemotherapy 2004;36(6):357-365
BACKGROUND: Although several molecular typing methods have been used to investigate C. albicans infections, there remains no "gold standard" method by which relatedness of C. albicans strains is determined. In this study, two DNA fingerprinting methods were compared for genotyping of clinical strains of C. albicans isolated from candidemic patients. MATERIALS AND METHODS: Twenty-nine strains of C. albicans isolated from various clinical specimens (14 from blood, 7 from catheter, 4 from respiratory tract secretion, and 4 from urine) of 14 candidemic patients were analyzed. Primer 1245 and 1246 were employed for IR PCR and Southern blot hybridization method was used for C2 fingerprinting, with Ca3 and C1 as primers, after the fragmentation of DNA with EcoR1 RESULTS: IR PCR method separated 29 isolates into 9 (1245 primer), 7 (1246 primer) and 14 (combination of two primers) types, whereas C1 fingerprinting identified 16 different types. By combining the IR PCR and C1 fingerprinting methods, total of 16 different genotypes were identified among 29 isolates from 14 patients, which is the same result obtained by the C1 fingerprinting only. Using both methods, blood and non-blood isolates from each patient produced identical genotypes for 10 patients and different genotypes for 1 patient. In three patients, isolates from blood and other site of each patient showed identical patterns by IR PCR fingerprinting, but appeared different (n=1) or similar (n=2) by C1 fingerprinting. Overall, for 87% (13/15) of patients, isolates collected from catheter (6 of 7 patients), urine (4 of 4 patients), or respiratory (3 of 4 patients) were identical or similar to the corresponding blood isolates. CONCLUSION: Our study shows that C1 fingerprinting method is more discriminatory than IR PCR for the molecular typing of C. albicans isolates. For the majority of patients, blood and other site isolates had identical or similar genotypes.
Blotting, Southern
;
Candida albicans*
;
Candida*
;
Candidemia
;
Catheters
;
Dermatoglyphics
;
DNA Fingerprinting*
;
DNA*
;
Genotype
;
Humans
;
Molecular Typing
;
Polymerase Chain Reaction*
;
Respiratory System
3.DNA Fingerprinting of Candida albicans Strains Isolated from Candidemic Patients by Polymerase Chain Reaction and Southern Hybridization Methods.
Ju Yeoul PARK ; Jong Hee SHIN ; Sung Jin YANG ; Bong Joon OH ; Duck CHO ; Seong Jung KEE ; Myung Gun SHIN ; Soon Pal SUH ; Dong Wook RYANG
Infection and Chemotherapy 2004;36(6):357-365
BACKGROUND: Although several molecular typing methods have been used to investigate C. albicans infections, there remains no "gold standard" method by which relatedness of C. albicans strains is determined. In this study, two DNA fingerprinting methods were compared for genotyping of clinical strains of C. albicans isolated from candidemic patients. MATERIALS AND METHODS: Twenty-nine strains of C. albicans isolated from various clinical specimens (14 from blood, 7 from catheter, 4 from respiratory tract secretion, and 4 from urine) of 14 candidemic patients were analyzed. Primer 1245 and 1246 were employed for IR PCR and Southern blot hybridization method was used for C2 fingerprinting, with Ca3 and C1 as primers, after the fragmentation of DNA with EcoR1 RESULTS: IR PCR method separated 29 isolates into 9 (1245 primer), 7 (1246 primer) and 14 (combination of two primers) types, whereas C1 fingerprinting identified 16 different types. By combining the IR PCR and C1 fingerprinting methods, total of 16 different genotypes were identified among 29 isolates from 14 patients, which is the same result obtained by the C1 fingerprinting only. Using both methods, blood and non-blood isolates from each patient produced identical genotypes for 10 patients and different genotypes for 1 patient. In three patients, isolates from blood and other site of each patient showed identical patterns by IR PCR fingerprinting, but appeared different (n=1) or similar (n=2) by C1 fingerprinting. Overall, for 87% (13/15) of patients, isolates collected from catheter (6 of 7 patients), urine (4 of 4 patients), or respiratory (3 of 4 patients) were identical or similar to the corresponding blood isolates. CONCLUSION: Our study shows that C1 fingerprinting method is more discriminatory than IR PCR for the molecular typing of C. albicans isolates. For the majority of patients, blood and other site isolates had identical or similar genotypes.
Blotting, Southern
;
Candida albicans*
;
Candida*
;
Candidemia
;
Catheters
;
Dermatoglyphics
;
DNA Fingerprinting*
;
DNA*
;
Genotype
;
Humans
;
Molecular Typing
;
Polymerase Chain Reaction*
;
Respiratory System