Primary systemic mycoses General  These are primary fungal infections. They don ’ t require risk factors to occur. They affect normal and compromised.

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Primary systemic mycoses General  These are primary fungal infections. They don ’ t require risk factors to occur. They affect normal and compromised subjects  They starts as a respiratory disease and if not cured, they disseminate to other body sites like, skin bone and subcutaneous tissues, central nervous system, bone marrow … etc  Contracted by inhalation of fungal elements in dust  Symptom include flu signs initially, then fever, cough, chest pain, and, loss of weight, night sweats-other signs of sites they disseminate  Common in north America and to a lesser extend south America not common in other part of the world  Etiologies are dimorphic fungi. In nature found in soil of restricted habitats  Drugs of choice for treatment: amphotericin B, liposomal amphotericin, voriconazole, caspofungin, other new antifungal  They include: Blastomycosis, Hsitoplasmosis, Coccidiodomycosis, Paracocidiomycosis

Blastomycosis The general statements about the primary systemic apply to this infection The pulmonary form is progressive, and if not treated it disseminates to skin, subcutaneous tissue, bone, central nervous system (CNS). Etiology: Blastomyces dermatitidis Dimorphic, imperfect, moniliaceous fungus It is mold in nature and in culture at ≤30 C. But yeasts in human body and culture at 37 c The mold is white with septate hyphae and lateral unicellular conidia the yeasts cells are large 8-15 um in diameter with broad –base attachment of bud to mother cell In nature, it is present in soil rich in organic matter The perfect stage of the fungus has been discovered and it is an ascomycete reproduce sexually forming ascospores. Named, Ajellomyces dermatitdis

Laboratory diagnosis specimens: respiratory (sputum, bronchoscopic) or biopsy tissue from site, blood for serology Direct microscopy: yeast cells with broad – base budding Culture on SDA, blood agar, BHI-A at ≤30 c---- mold at 37 c ---yeasts Serology: test for AB using known Ag (blastomycin) Methods: ID, CIE, complement fixation (CF) there is cross reactivity with others Treatment: as mentioned in the general statements

Histoplasmosis (cave Disease) This is an intracellular infection of the reticuloendothelial system (RES) Starts as respiratory-could be self – limiting The pulmonary form similar to tuberculosis-there is caseation and fibrosis. Disseminates to RES (liver spleen, bone marrow – macrophages) Seen more in USA reported from other parts of the world Etiology: Histoplasma capsulatum Dimorphic, imperfect, moniliaceous fungus Mold in nature and in culture at ≤ 30C yeast in human body and in culture at 37 c There are two varieties of the species, differing mainly in the yeast phase and having same mold phase. These varities are: H. capsulatum; has small (2-3 x 3-4 um) oval yeast cells causes the usual histoplasmosis H. cap. Var. duboisii; has large yeast cells (7-5 um), causes African histoplasmosis. t

The mold phase has white colonies, septat hyphae, produces two types of conidia: Tuberculated macroconidia (8-14 um), and smooth Microconidia (2-5 um) The natural habitat of the fungus is specific soils rich in animal excreta especially bat guano and droppings of certain birds. Because caves harbor bats- thus called “ cave disease ” The perfect stage of the fungus has been known; it is ascomycete producing ascospores sexually called Ajellomyces capsulatus

Laboratory diagnosis: specimen: respiratory, biopsy tissue of affected site, blood, bone marrow Direct microscopy: intracellular yeast cells in macrophages- small for var. capsul, and large for var. duboisii Culture: on SDA, BHI-A, BHI-A-blood (biphasic medium) incubate at 30 c and 37 c. slow growth for primary isolation-may takes weeks Serology: test for AB in patient serum using known Ag (Histoplasmin Ag, H and M Ags) using ID, CIE, CF. there is cross reactivity Treatment: As mentioned in the general statements.

Coccidioidomycosis (valley fever) Clinical: Starts as respiratory could be self limiting If pulmonary not cured-it may disseminate Endemic in southwestern USA (Southern California, and Arizona) where it is known as valley fever, children summer Sickness and adults flue Rarely seen out of America Etiology Coccidioides immitis Dimorphic imperfect moniliaceous fungus Mold in nature and in culture at ≤ 30 c The other phase is spherules with endospores in human body and in modified converse medium at 37 c The natural habitat of the fungus in soil, in rodent-burrows or around them in hot dry deserts

The mold phase has white colonies with septat hyphae. It produces berrel-shaped arthrospores (2.5 -4x 3-6 um) that alternate with disjunctor cells The spherule phase will have large spherules (30-60 um) upon maturity with endospores Laboratory diagnosis specimens: respiratory (sputum, bronchoscopic), biopsy tissue from site of infection, blood for serology) Direct microscopy presence of spherules, mature spherules with endospores Culture grows readily on SDA at room temperature or 37 c on modified converse medium at 37 c and reduced oxygen the spherules will be produced readily

Serology Test for AB in patient serum using known AG (coccidioidin Ag) Methods include CF tube precipitin test ID and CIE Serology Is good rising titers---infection Declining titers ---remission Treatment,, As general statement

Paracoccidioidomycosis Southamerican blastomycosis Additional symptom: ulcers in buccal mucosa and lymphoadenopathy The infection is more seen in South American countries )brazil, Veneziuella, Argentina, chill, --etc) it is rarely seen elsewhere Etiology: paracocccidioides brasiliensisi Dimorphic, imperfect, moniliaceous fungus It is mold in nature and in culture at ≤ 30 c, and large yeast in human body and in culture at 37 c on blood agar The mold grows as white colonies with septat hyphae having chlamydospores and lateral unicellular conidia The yeasts phase has large yeast cells (some up to 30 um in diameter) with multiple nuclei and multiple buds; known as mariner’s wheel cell or Mickey mouse cell

Laboratory diagnosis Specimens respiratory, aspirates, ulcerative material, biopsy tissue from site of infection, blood for serology Direct microscopy: presence of budding yeast cells some large with multiple nuclei and buds, marriner ’ s wheels cells / Mickey mouse cells Culture on SDA incubate at room temperature to grow mold phase, and blood agar at 37 c to grow the yeast phase Serology: test for AB Treatment: as in general statement. Mild cases can be treated with sulphonamides