Chemical and immunochemical characterization of limulus factor G-activating substance of Candida spp

Chemical and immunochemical characterization of limulus factor G-activating substance of Candida spp

Abstract The limulus test is a well-established method for the diagnosis of both Gram (−) sepsis and invasive fungal infection. To diagnose deep-seated fungal infections, a (1→3)-β-d-glucan-specific chromogenic kit (Fungitec G test MK) has been developed and applied clinically. It is suggested that...

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Bibliographic Details
Published in:FEMS immunology and medical microbiology Vol. 24; no. 4; pp. 411 - 420
Main Authors: Uchiyama, Michiharu, Ohno, Naohito, Miura, Noriko N., Adachi, Yoshiyuki, Aizawa, Maki W., Tamura, Hiroshi, Tanaka, Shigenori, Yadomae, Toshiro
Format: Journal Article
Language:English
Published: Oxford, UK Blackwell Publishing Ltd 01-07-1999
Blackwell
Subjects:
Biological and medical sciences
Candida
Candida - chemistry
Cell wall
Chemical Fractionation
Diagnosis
Enzyme-Linked Immunosorbent Assay
Fungal infection
Glucans - analysis
Glucans - chemistry
Human mycoses
Infectious diseases
Limulus Test
Mannans - analysis
Medical sciences
Mycoses
Mycotic sepsis
Nuclear Magnetic Resonance, Biomolecular
Solubility
β‐Glucan
Limulus test
Diagnosis
β-Glucan
Fungal infection
Cell wall
Human
Candidiasis
Yeast
Mycosis
Systemic
Mannan
Fungi
Infection
Glucan
Candida
Fungi Imperfecti
Limulus lysate assay
Thallophyta
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Summary:Abstract The limulus test is a well-established method for the diagnosis of both Gram (−) sepsis and invasive fungal infection. To diagnose deep-seated fungal infections, a (1→3)-β-d-glucan-specific chromogenic kit (Fungitec G test MK) has been developed and applied clinically. It is suggested that the limulus reactive substance was released from the fungi to the blood, however, its chemical properties were not precisely examined in detail because of the limited quantity available. In this study, we used chemically defined liquid medium to culture Candida spp. and collected the water soluble fraction, CAWS. The yield of CAWS was circa 100 mg/l, independent of the strain of Candida. CAWS reacted with limulus factor G (Fungitec G test MK) at concentrations as low as 100 ng/ml. Limulus factor G reactivity of CAWS was sensitive to (1→3)-β-glucanase, zymolyase and was, at least in part, bound to ConA-agarose. The ConA-bound fraction also reacted with anti-β-glucan antibody. CAWS is mainly composed of mannan and (1→6)-β-glucan, in addition to protein, assessed by 1H-NMR spectroscopy. CAWS also reacted with typing sera of Candida spp., specific for cell wall mannan. Chemical, immunochemical and biochemical analyses of CAWS strongly suggested that the limulus factor G-activating substance was a mannan-β-glucan complex, present within the architecture of the yeast cell wall.
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ISSN:0928-8244
1574-695X
DOI:10.1111/j.1574-695X.1999.tb01313.x