Adverse Human Health Effects Associated with Molds in the Indoor
Environment Copyright © 2002 American College of Occupational and
Environmental Medicine
In recent years, the growth of molds in home, school, and
office environments has been cited as the cause of a wide variety of
human ailments and disabilities. So-called "toxic mold" has become a
prominent topic in the lay press and is increasingly the basis for
litigation when individuals, families, or building occupants believe
they have been harmed by exposure to indoor molds. This evidence-based
statement from the American College of Occupational and Environmental
Medicine (ACOEM) discusses the state of scientific knowledge as to the
nature of fungal-related illnesses while emphasizing the possible
relationships to indoor environments. Particular attention is given to
the possible health effects of mycotoxins, which give rise to much of
the concern and controversy surrounding indoor molds. Food-borne
exposures, methods of exposure assessment, and mold remediation
procedures are beyond the scope of this paper. 
The fungi are eukaryotic, unicellular, or multicellular
organisms that, because they lack chlorophyll, are dependent upon
external food sources. Fungi are ubiquitous in all environments and play
a vital role in the Earth's ecology by decomposing organic matter.
Familiar fungi include yeasts, rusts, smuts, mushrooms, puffballs, and
bracket fungi. Many species of fungi live as commensal organisms in or
on the surface of the human body. "Mold" is the common term for
multicellular fungi that grow as a mat of intertwined microscopic
filaments (hyphae). Exposure to molds and other fungi and their spores
is unavoidable except when the most stringent of air filtration,
isolation, and environmental sanitation measures are observed, eg, in
organ transplant isolation units.
Molds and other fungi may adversely affect human health through
three processes: 1) allergy; 2) infection; and 3) toxicity. One can
estimate that about 10% of the population has allergic antibodies to
fungal antigens. Only half of these, or 5%, would be expected to show
clinical illness. Furthermore, outdoor molds are generally more abundant
and important in airway allergic disease than indoor molds ˆ… leaving
the latter with an important, but minor overall role in allergic airway
disease. Allergic responses are most commonly experienced as allergic
asthma or allergic rhinitis ("hay fever"). A rare, but much more serious
immune-related condition, hypersensitivity pneumonitis (HP), may follow
exposure (usually occupational) to very high concentrations of fungal
(and other microbial) proteins.
Most fungi generally are not pathogenic to healthy humans. A
number of fungi commonly cause superficial infections involving the feet
(tinea pedis), groin (tinea cruris), dry body skin (tinea corporus), or
nails (tinea onchomycosis). A very limited number of pathogenic fungi
ˆ… such as Blastomyces, Coccidioides, Cryptococcus, and Histoplasma ˆ…
infect non-immunocompromised individuals. In contrast, persons with
severely impaired immune function, eg, cancer patients receiving
chemotherapy, organ transplant patients receiving immunosuppressive
drugs, AIDS patients, and patients with uncontrolled diabetes, are at
significant risk for more severe opportunistic fungal infection.
Some species of fungi, including some molds, are known to be
capable of producing secondary metabolites, or mycotoxins, some of which
find a valuable clinical use, eg, penicillin, cyclosporine. Serious
veterinary and human mycotoxicoses have been documented following
ingestion of foods heavily overgrown with molds. In agricultural
settings, inhalation exposure to high concentrations of mixed organic
dusts ˆ… which include bacteria, fungi, endotoxins, glucans, and
mycotoxins ˆ… is associated with organic dust toxic syndrome, an acute
febrile illness. The present alarm over human exposure to molds in the
indoor environment derives from a belief that inhalation exposures to
mycotoxins cause numerous and varied, but generally nonspecific,
symptoms. Current scientific evidence does not support the proposition
that human health has been adversely affected by inhaled mycotoxins in
the home, school, or office environment.
Allergy and other hypersensitivity reactions
Allergic and other hypersensitivity responses to indoor molds
may be immunoglobulin E (IgE) or immunoglobulin G (IgG) mediated, and
both types of response are associated with exposure to indoor molds.
Uncommon allergic syndromes, allergic bronchopulmonary aspergillosis
(ABPA), and allergic fungal sinusitus (AFS), are briefly discussed for
completeness, although indoor mold has not been suggested as a
particular risk factor in the etiology of either.-
Immediate hypersensitivity: The most common form of
hypersensitivity to molds is immediate type hypersensitivity or
IgE-mediated "allergy" to fungal proteins. This reactivity can lead to
allergic asthma or allergic rhinitis that is triggered by breathing in
mold spores or hyphal fragments. Residential or office fungal exposures
may be a substantial factor in an individual's allergic airway disease
depending on the subject's profile of allergic sensitivity and the
levels of indoor exposures. Individuals with this type of mold allergy
are "atopic" individuals, ie, have allergic asthma, allergic rhinitis,
or atopic dermatitis and manifest allergic (IgE) antibodies to a wide
range of environmental proteins among which molds are only one
participant. These individuals generally will have allergic reactivity
against other important indoor and outdoor allergens such as animal
dander, dust mites, and weed, tree, and grass pollens. Among the fungi,
the most important indoor allergenic molds are Penicillium and
Aspergillus species.1 Outdoor molds, eg, Cladosporium and Alternaria, as
well as pollens, can often be found at high levels indoors if there is
access for outdoor air (eg, open windows).
About 40% of the population are atopic and express high levels of allergic antibodies to inhalant allergens. Of these, 25%, or 10% of the population, have allergic antibodies to common inhalant molds.2 Since about half of persons with allergic antibodies will express clinical disease from those antibodies, about 5% of the population is predicted to have, at some time, allergic symptoms from molds. While indoor molds are well-recognized allergens, outdoor molds are more generally important.
A growing body of literature associates a variety of diagnosable respiratory illnesses (asthma, wheezing, cough, phlegm, etc.), particularly in children, with residence in damp or water-damaged homes (see reviews 3-5). Recent studies have documented increased inflammatory mediators in the nasal fluids of persons in damp buildings, but found that mold spores themselves were not responsible for these changes.6,7 While dampness may indicate potential mold growth, it is also a likely indicator of dust mite infestation and bacterial growth. The relative contribution of each is unknown, but mold, bacteria, bacterial endotoxins, and dust mites can all play a role in the reported spectrum of illnesses, and can all be minimized by control of relative humidity and water intrusion.
-
Hypersensitivity pneumonitis (HP): HP results from
exaggeration of the normal IgG immune response against inhaled foreign
(fungal or other) proteins and is characterized by: 1) very high serum
levels of specific IgG proteins (classically detected in precipitin
tests performed as double diffusion tests); and 2) inhalation exposure
to very large quantities of fungal (or other) proteins.8 The resulting
interaction between the inhaled fungal proteins and fungal-directed cell
mediated and humoral (antibody) immune reactivity leads to an intense
local immune reaction recognized as HP. As opposed to immediate
hypersensitivity (IgE-mediated) reactions to mold proteins, HP is not
induced by normal or even modestly elevated levels of mold spores. Most
cases of HP result from occupational exposures, although cases have also
been attributed to pet birds, humidifiers, and heating, ventilating,
and air conditioning (HVAC) systems. The predominant organisms in the
latter two exposures are thermophilic Actinomyces, which are not molds
but rather are filamentous bacteria that grow at high temperatures
(116¬°F).
The presence of high levels of a specific antibody ˆ… generally demonstrated as the presence of precipitating antibodies ˆ… is required to initiate HP, but is not diagnostic of HP.9 More than half of the people who have occupational exposure to high levels of a specific protein have such precipitin antibodies, but do not have clinical disease.8 Many laboratories now measure IgG to selected antigens by using solid phase immunoassays, which are easier to perform and more quantitative than precipitin (gel diffusion) assays. However, solid phase IgG levels that are above the reference range do not carry the same discriminatory power as do results of a precipitin test, which requires much greater levels of antibody to be positive. Five percent of the normal population have levels above the reference value for any one tested material. Consequently, a panel of tests (eg, 10) has a high probability of producing a false-positive result. Screening IgG antibody titers to a host of mold and other antigens is not justified unless there is a reasonable clinical suspicion for HP and should not be used to screen for mold exposure.10
-
Uncommon allergic syndromes: Allergic bronchopulmonary
aspergillosis (ABPA) and allergic fungal sinusitis (AFS).11 These
conditions are unusual variants of allergic (IgE-mediated) reactions in
which fungi actually grow within the patient's airway. ABPA is the
classic form of this syndrome, which occurs in allergic individuals who
generally have airway damage from previous illnesses leading to
bronchial irregularities that impair normal drainage, eg,
bronchiectasis.12,13 Bronchial disease and old cavitary lung disease are
predisposing factors contributing to fungal colonization and the
formation of mycetomas. Aspergillus may colonize these areas without
invading adjacent tissues. Such fungal colonization is without adverse
health consequence unless the subject is allergic to the specific fungus
that has taken up residence, in which case there may be ongoing
allergic reactivity to fungal proteins released directly into the body.
Specific criteria have been recognized for some time for the diagnosis
of ABPA.14,15 As fungi other than Aspergillus may cause this condition,
the term "allergic bronchopulmonary mycosis" has been suggested.
It has more recently become appreciated that a similar process may affect the sinuses ˆ… allergic fungal sinusitis (AFS).16 This condition also presents in subjects who have underlying allergic disease and in whom, because of poor drainage, a fungus colonizes the sinus cavity. Aspergillus and Curvularia are the most common forms, although the number of fungal organisms involved continues to increase. As with ABPA, the diagnosis of AFS has specific criteria that should be used to make this diagnosis.17-19
Recommendations
Individuals with allergic airway disease should take steps to
minimize their exposure to molds and other airborne allergens, eg,
animal dander, dust mites, pollens. For these individuals, it is prudent
to take feasible steps that reduce exposure to aeroallergens and to
remediate sources of indoor mold amplification. Sensitized individuals
may need to keep windows closed, remove pets, use dust mite covers, use
high-quality vacuum cleaners, or filter outdoor air intakes to minimize
exposures to inhalant allergens. Humidification over 40% encourages
fungal and dust mite growth, so should be avoided. Where there is indoor
amplification of fungi, removal of the fungal source is a key measure
to be undertaken so as to decrease potential for indoor mold allergen
exposure.
ABPA and AFS are uncommon disorders while exposure is
ubiquitous to the fungal organisms involved. There is no evidence to
link specific exposures to fungi in home, school, or office settings to
the establishment of fungal colonization that leads to ABPA or AFS.
Once a diagnosis of HP is entertained in an appropriate
clinical setting and with appropriate laboratory support, it is
important to consider potential sources of inhaled antigen. If
evaluation of the occupational environment fails to disclose the source
of antigens, exposures in the home, school, or office should be
investigated. Once identified, the source of the mold or other inhaled
foreign antigens should be remediated.
Appropriate measures should be taken in industrial workplaces
to prevent mold growth, eg, in machining fluids and where stored organic
materials are handled such as in agricultural and grain processing
facilities. Engineering controls and personal protective equipment
should be used to reduce aerosol generation and minimize worker
exposures to aerosols.
Although it is not relevant to indoor mold exposure, it should
be mentioned that there is a belief among some health practitioners and
members of the public regarding a vague relationship between mold
colonization, molds in foods, and a ˆ£generalized mold hypersensitivity
state.ˆ§ The condition was originally proposed as the ˆ£Chronic Candida
Syndromeˆ§ or ˆ£Candida Hypersensitivity Syndrome,ˆ§ but now has been
generalized to other fungi. Adherents may claim that individuals are
ˆ£colonizedˆ§ with the mold(s) to which they are sensitized and that
they react to these endogenous molds as well as to exposures in foods
and other materials that contain mold products. The proposed
hypersensitivity is determined by the presence of any of a host of
non-specific symptoms plus an elevated (or even normal) level of IgG to
any of a host of molds. The claim of mold colonization is generally not
supported with any evidence, eg, cultures or biopsies, to demonstrate
the actual presence of fungi in or on the subject. Instead, proponents
often claim colonization or infection based on the presence of a wide
variety of nonspecific symptoms and antibodies detected in serologic
tests that represent no more than past exposure to normal environmental
fungi. The existence of this disorder is not supported by reliable
scientific data (20, 21).
Infection
An overview of fungi as human pathogens follows. Exposure to
molds indoors is generally not a specific risk factor in the etiology of
mycoses except under specific circumstances as discussed below for
individual types of infection.
- Serious fungal infections: A very limited number of pathogenic fungi such as Blastomyces, Coccidioides, Cryptococcus, and Histoplasma infect normal subjects and may cause a fatal illness. However, fungal infections in which there is deep tissue invasion are primarily restricted to severely immunocompromised subjects, eg, patients with lymphoproliferative disorders including acute leukemia, cancer patients receiving intense chemotherapy, or persons undergoing bone marrow or solid transplantation who get potent immunosuppressive drugs.22 Uncontrolled diabetics and persons with advanced AIDS are also at increased risk. Concern is greatest when patients are necessarily in the hospital during their most severe immunocompromise, at which time intense measures are taken to avoid fungal, bacterial, and viral infection.23 Outside the hospital, fungi, including Aspergillus, are so ubiquitous that few recommendations can be made beyond avoidance of known sources of indoor and outdoor amplification, including indoor plants and flowers because vegetation is a natural fungal growth medium.24,25 Candida albicans is a ubiquitous commensal organism on humans that becomes an important pathogen for immunocompromised subjects. However, it and other environmental fungi discussed above that are pathogens in normals as well (eg, Cryptococcus associated with bird droppings, Histoplasma associated with bat droppings, Coccidioides endemic in the soil in the southwest US) are not normally found growing in the office or residential environment, although they can gain entry from outdoors. Extensive guidelines for specific immunocompromised states can be found at the Centers for Disease Control and Prevention (CDC) web site at www.cdc.gov.
-
Superficial fungal infections: In contrast to serious
internal infections with fungi, superficial fungal infections on the
skin or mucosal surfaces are extremely common in normal subjects. These
superficial infections include infection of the feet (tinea pedis),
nails (tinea onychomycosis), groin (tinea cruris), dry body skin (tinea
corporis), and infection of the oral or vaginal mucosa. Some of the
common organisms involved, eg, Trychophyton rubrum, can be found growing
as an indoor mold. Others, such as Microsprum canis and T.
mentagrophytes can be found on indoor pets (eg, dogs, cats, rabbits, and
guinea pigs). As a common commensal on human mucosal surfaces, C.
albicans can be cultured from more than half of the population that has
no evidence of active infection. C. albicans infections are particularly
common when the normally resident microbial flora at a mucosal site are
removed by antibiotic use. Local factors such as moisture in shoes or
boots and in body creases and loss of epithelial integrity are important
in development of superficial fungal infections.
Pityriasis (Tinea) versicolor is a chronic asymptomatic infection of the most superficial layers of the skin due to Pityriasis ovale (also known as P. orbiculare and Malassesia furfur) manifest by patches of skin with variable pigmentation. This is not a contagious condition and thus is unrelated to exposures, but represents the overgrowth of normal cutaneous fungal flora under favorable conditions.=
Recommendations
- Only individuals with the most severe forms of immunocompromise need be concerned about the potential for opportunistic fungal infections. These individuals should be advised to avoid recognizable fungal reservoirs including, but not limited, to indoor environments where there is uncontrolled mold growth. Outdoor areas contaminated by specific materials such as pigeon droppings should be avoided as well as nearby indoor locations where those sources may contaminate the intake air.
- Individuals with M. canis and T. mentagrophytes infections should have their pets checked by a veterinarian. No other recommendations are warranted relative to home, school, or office exposures in patients with superficial fungal infections.
Toxicity
Mycotoxins are ˆ£secondary metabolitesˆ§ of fungi, which is to
say mycotoxins are not required for the growth and survival of the
fungal species (ˆ£toxigenic speciesˆ§) that are capable of producing
them. The amount (if any) and type of mycotoxin produced is dependent on
a complex and poorly understood interaction of factors that probably
include nutrition, growth substrate, moisture, temperature, maturity of
the fungal colony, and competition from other microorganisms.26-30
Additionally, even under the same conditions of growth, the profile and
quantity of mycotoxins produced by toxigenic species can vary widely
from one isolate to another.31-34 Thus, it does not necessarily follow
from the mere presence of a toxigenic species that mycotoxins are also
present.35-38
When produced, mycotoxins are found in all parts of the fungal
colony, including the hyphae, mycelia, spores, and the substrate on
which the colony grows. Mycotoxins are relatively large molecules that
are not significantly volatile;39,40 they do not evaporate or
ˆ£off-gasˆ§ into the environment, nor do they migrate through walls or
floors independent of a particle. Thus, an inhalation exposure to
mycotoxins requires generation of an aerosol of substrate, fungal
fragments, or spores. Spores and fungal fragments do not pass through
the skin, but may cause irritation if there is contact with large
amounts of fungi or contaminated substrate material.41 In contrast,
microbial volatile organic compounds (MVOCs) are low molecular weight
alcohols, aldehydes, and ketones.42 Having very low odor thresholds,
MVOCs are responsible for the musty, disagreeable odor associated with
mold and mildew and they may be responsible for the objectionable taste
of spoiled foods.42,43
Most descriptions of human and veterinary poisonings from molds
involve eating moldy foods.41,43-46 Acute human intoxications have also
been attributed to inhalation exposures of agricultural workers to
silage or spoiled grain products that contained high concentrations of
fungi, bacteria, and organic debris with associated endotoxins, glucans,
and mycotoxins.47,48 Related conditions including ˆ£pulmonary
mycotoxicosis,ˆ§ ˆ£grain fever,ˆ§ and others are referred to more
broadly as ˆ£organic dust toxic syndromeˆ§ (ODTS).49 Exposures
associated with ODTS have been described as a ˆ£fogˆ§ of particulates50
or an initial ˆ£thick airborne dustˆ§ that ˆ£worsened until it was no
longer possible to see across the room.ˆ§51 Total microorganism counts
have ranged from 105-109 per cubic meter of air52 or even 109-1010
spores per cubic meter,53,54 extreme conditions not ordinarily
encountered in the indoor home, school, or office environment.
ˆ£Sick building syndrome,ˆ§ or ˆ£non-specific building-related
illness,ˆ§ represents a poorly defined set of symptoms (often sensory)
that are attributed to occupancy in a building. Investigation generally
finds no specific cause for the complaints, but they may be attributed
to fungal growth if it is found. The potential role of
building-associated exposure to molds and associated mycotoxins has been
investigated, particularly in instances when Stachybotrys chartarum
(aka Stachybotrys atra) was identified.55-58 Often referred to in the
lay press by the evocative, but meaningless terms, ˆ£toxic moldˆ§ or
ˆ£fatal fungus,ˆ§ S. chartarum elicits great concern when found in
homes, schools, or offices, although it is by no means the only mold
found indoors that is capable of producing mycotoxins.35,36,59,60 Recent
critical reviews of the literature35,61-67 concluded that indoor
airborne levels of microorganisms are only weakly correlated with human
disease or building-related symptoms and that a causal relationship has
not been established between these complaints and indoor exposures to S.
chartarum.
A 1993-1994 series of cases of pulmonary hemorrhage among
infants in Cleveland, Ohio, led to an investigation by the CDC and
others. No causal factors were suggested initially,68 but eventually
these same investigators proposed that the cause had been exposures in
the home to S. chartarum and suggested that very young infants might be
unusually vulnerable.69-71 However, subsequent detailed re-evaluations
of the original data by CDC and a panel of experts led to the conclusion
that these cases, now called "acute idiopathic pulmonary hemorrhage in
infants,ˆ§72 had not been causally linked to S. chartarum exposure.73
If mycotoxins are to have human health effects, there must be
an actual presence of mycotoxins, a pathway of exposure from source to
susceptible person, and absorption of a toxic dose over a sufficiently
short period of time. As previously noted, the presence of mycotoxins
cannot be presumed from the mere presence of a toxigenic species. The
pathway of exposure in home, school, and office settings may be either
dermal (eg, direct contact with colonized building materials) or
inhalation of aerosolized spores, mycelial fragments, or contaminated
substrates. Because mycotoxins are not volatile, the airborne pathway
requires active generation of that aerosol. For toxicity to result, the
concentration and duration of exposure must be sufficient to deliver a
toxic dose. What constitutes a toxic dose for humans is not known at the
present time, but some estimates can be made that suggest under what
circumstances an intoxication by the airborne route might be feasible.
Experimental data on the in vivo toxicity of mycotoxins are
scant. Frequently cited are the inhalation LC50 values determined for
mice, rats, and guinea pigs exposed for 10 minutes to T-2 toxin, a
trichothecene mycotoxin produced by Fusarium spp.74,75 Rats were most
sensitive in these studies, but there was no mortality in rats exposed
to 1.0 mg T-2 toxin/m3. No data were found on T-2 concentrations in
Fusarium spores, but another trichothecene, satratoxin H, has been
reported at a concentration of 1.0 x 10-4 ng/spore in a ˆ£highly toxicˆ§
S. chartarum strain s. 72.31 To provide perspective relative to T-2
toxin, 1.0 mg satratoxin H/m3 air would require 1010 (ten billion) of
these s. 72 S. chartarum spores/m3.
In single-dose in vivo studies, S. chartarum spores have been
administered intranasally to mice31 or intratracheally to rats.76,77
High doses (30 x 106 spores/kg and higher) produced pulmonary
inflammation and hemorrhage in both species. A range of doses were
administered in the rat studies and multiple, sensitive indices of
effect were monitored, demonstrating a graded dose response with 3 x 106
spores/kg being a clear no-effect dose. Airborne S. chartarum spore
concentrations that would deliver a comparable dose of spores can be
estimated by assuming that all inhaled spores are retained and using
standard default values for human subpopulations of particular
interest78 ˆ very small infants,¬† school-age children,¬†¬† and
adults.    The no-effect dose in rats (3 x 106 spores/kg) corresponds
to continuous 24-hour exposure to 2.1 x 106 spores/m3 for infants, 6.6 x
106 spores/m3 for a school-age child, or 15.3 x 106 spores/m3 for an
adult.
That calculation clearly overestimates risk because it ignores
the impact of dose rate by implicitly assuming that the acute toxic
effects are the same whether a dose is delivered as a bolus
intratracheal instillation or gradually over 24 hours of inhalation
exposure. In fact, a cumulative dose delivered over a period of hours,
days, or weeks is expected to be less acutely toxic than a bolus dose,
which would overwhelm detoxification systems and lung clearance
mechanisms. If the no-effect 3 x 106 spores/kg intratracheal bolus dose
in rats is regarded as a 1-minute administration (3 x 106
spores/kg/min), achieving the same dose rate in humans (using the same
default assumptions as previously) would require airborne concentrations
of 3.0 x 109 spores/m3 for an infant, 9.5 x 109 spores/m3 for a child,
or 22.0 x 109 spores/m3 for an adult.
In a repeat-dose study, mice were given intranasal treatments
twice weekly for three weeks with ˆ£highly toxicˆ§ s. 72 S. chartarum
spores at doses of 4.6 x 106 or 4.6 x 104 spores/kg (cumulative doses
over three weeks of 2.8 x 107 or 2.8 x 105 spores/kg).79 The higher dose
caused severe inflammation with hemorrhage, while less severe
inflammation, but no hemorrhage was seen at the lower dose of s. 72
spores. Using the same assumptions as previously (and again ignoring
dose-rate implications), airborne S. chartarum spore concentrations that
would deliver the non-hemorrhagic cumulative three-week dose of 2.8 x
105 spores/kg can be estimated as 9.4 x 103 spores/m3 for infants, 29.3 x
103 spores/m3 for a school-age child, and 68.0 x 103 spores/m3 for
adults (assuming exposure for 24 hours per day, 7 days per week, and
100% retention of spores).
The preceding calculations suggest lower bound estimates of
airborne S. chartarum spore concentrations corresponding to essentially
no-effect acute and subchronic exposures. Those concentrations are not
infeasible, but they are improbable and inconsistent with reported spore
concentrations. For example, in data from 9,619 indoor air samples from
1,717 buildings, when S. chartarum was detected in indoor air (6% of
the buildings surveyed) the median airborne concentration was 12 CFU/m3
(95% CI 12 to 118 CFU/m3).80
Recommendations
- The presence of toxigenic molds within a home, school, or office environment should not by itself be regarded as demonstrating that mycotoxins were present or that occupants of that environment absorbed a toxic dose of mycotoxins.
- Indoor air samples with contemporaneous outdoor air samples can assist in evaluating whether or not there is mold growth indoors; air samples may also assist in evaluating the extent of potential indoor exposure. Bulk, wipe, and wall cavity samples may indicate the presence of mold, but do not contribute to characterization of exposures for building occupants.
- After the source of moisture that supports mold growth has been eliminated, active mold growth can be eliminated. Colonized porous materials, eg, clothing or upholstery, can be cleaned using appropriate routine methods, eg, washing or dry cleaning clothing, and need not be discarded unless cleaning fails to restore an acceptable appearance.
- When patients associate health complaints with mold exposure, treating physicians should evaluate all possible diagnoses, including those unrelated to mold exposure, ie, consider a complete appropriate differential diagnosis for the patientˆ¢s complaints. To the extent that signs and symptoms are consistent with immune-mediated disease, immune mechanisms should be investigated.
- The possibility of a mycotoxicosis as an explanation for specific signs and symptoms in a residential or general office setting should be entertained only after accepted processes that are recognized to occur have been appropriately excluded and when mold exposure is known to be uncommonly high. If a diagnosis of mycotoxicosis is entertained, specific signs and symptoms ascribed to mycotoxins should be consistent with the potential mycotoxins present and their known biological effects at the potential exposure levels involved.
Summary
Molds are common and important allergens. About 5% of
individuals are predicted to have some allergic airway symptoms from
molds over their lifetime. However, it should be remembered that molds
are not dominant allergens and that the outdoor molds, rather than
indoor ones, are the most important. For almost all allergic
individuals, the reactions will be limited to rhinitis or asthma;
sinusitis may occur secondarily due to obstruction. Rarely do sensitized
individuals develop uncommon conditions such as ABPA or AFS. To reduce
the risk of developing or exacerbating allergies, mold should not be
allowed to grow unchecked indoors. When mold colonization is discovered
in the home, school, or office, it should be remediated after the source
of the moisture that supports its growth is identified and eliminated.
Authoritative guidelines for mold remediation are available.81-83
Fungi are rarely significant pathogens for humans. Superficial
fungal infections of the skin and nails are relatively common in normal
individuals, but those infections are readily treated and generally
resolve without complication. Fungal infections of deeper tissues are
rare and in general are limited to persons with severely impaired immune
systems. The leading pathogenic fungi for persons with nonimpaired
immune function, Blastomyces, Coccidioides, Cryptococcus, and
Histoplasma, may find their way indoors with outdoor air, but normally
do not grow or propagate indoors. Due to the ubiquity of fungi in the
environment, it is not possible to prevent immune-compromised
individuals from being exposed to molds and fungi outside the confines
of hospital isolation units.
Some molds that propagate indoors may, under some conditions,
produce mycotoxins that can adversely affect living cells and organisms
by a variety of mechanisms. Adverse effects of molds and mycotoxins have
been recognized for centuries following ingestion of contaminated
foods. Occupational diseases are also recognized in association with
inhalation exposure to fungi, bacteria, and other organic matter,
usually in industrial or agricultural settings. Molds growing indoors
are believed by some to cause building-related symptoms. Despite a
voluminous literature on the subject, the causal association remains
weak and unproven, particularly with respect to causation by mycotoxins.
One mold in particular, Stachybotrys chartarum, is blamed for a diverse
array of maladies when it is found indoors. Despite its well-known
ability to produce mycotoxins under appropriate growth conditions, years
of intensive study have failed to establish exposure to S. chartarum in
home, school, or office environments as a cause of adverse human health
effects. Levels of exposure in the indoor environment, dose-response
data in animals, and dose-rate considerations suggest that delivery by
the inhalation route of a toxic dose of mycotoxins in the indoor
environment is highly unlikely at best, even for the hypothetically most
vulnerable subpopulations.
Mold spores are present in all indoor environments and cannot
be eliminated from them. Normal building materials and furnishings
provide ample nutrition for many species of molds, but they can grow and
amplify indoors only when there is an adequate supply of moisture.
Where mold grows indoors there is an inappropriate source of water that
must be corrected before remediation of the mold colonization can
succeed. Mold growth in the home, school, or office environment should
not be tolerated because mold physically destroys the building materials
on which it grows, mold growth is unsightly and may produce offensive
odors, and mold is likely to sensitize and produce allergic responses in
allergic individuals. Except for persons with severely impaired immune
systems, indoor mold is not a source of fungal infections. Current
scientific evidence does not support the proposition that human health
has been adversely affected by inhaled mycotoxins in home, school, or
office environments.
Acknowledgments
Acknowledgments This ACOEM statement was prepared by Bryan D.
Hardin, PhD, Bruce J. Kelman, PhD, DABT, and Andrew Saxon, MD, under the
auspices of the ACOEM Council on Scientific Affairs. It was
peer-reviewed by the Council and its committees, and was approved by the
ACOEM Board of Directors on October 27, 2002. Dr. Hardin is the former
Deputy Director of NIOSH, Assistant Surgeon General (Retired), and
Senior Consultant to Global Tox, Inc, where Dr. Kelman is a Principal.
Dr. Saxon is Professor of Medicine at the School of Medicine, University
of California at Los Angeles.
  5th percentile body weight for 1-month-old male infants,
3.16 kg; respiratory rate for infants under 1 year of age, 4.5 m3/day78
   50th percentile body weight for 6-year-old boys, 22 kg; respiratory
rate for children age 6-9, 10.0 m3/day78     50th percentile body
weight for men aged 25-34 years, 77.5 kg; respiratory rate for men age
19-65, 15.2 m3/day78
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Allergens. In: Middleton E, Jr et al, eds. Allergy: Principles and
Practice. St. Louis: Mosby Co.; 1998:367-403.
2. Horner WE, et al. Fungal allergens. Clin Microbiol Rev. 1995;8:161-79.
3. Billings CG, Howard P. Damp housing and asthma. Monaldi Arch Chest Dis. 1998;53:43-9.
4. Burr ML. Health effects of indoor molds. Rev Environ Health. 2001;16:97-103.
5. Macher J. Health effects of bioaerosols. In: Macher J, ed. Bioaerosols: assessment and control. Cincinnati, OH: American Conference of Governmental Industrial Hygienists, 1999:3-1 to -12.
6. Purokivi MK, et al. Changes in pro-inflammatory cytokines in association with exposure to moisture-damaged building microbes. Eur Respir J. 2001;18:951-8.
7. Roponen M, et al. Fungal spores as such do not cause nasal inflammation in mold exposure. Inhal Toxicol. 2002;14:541-9.
8. Fink J, Zacharisen MC. Hypersensitivity Pneumonitis. In: Middleton E, Jr. et al, eds. Allergy: Principles and Practice. St. Louis: Mosby Co.; 1998:994-1004.
9. Flaherty DK, et al. Multilaboratory comparison of three immunodiffusion methods used for the detection of precipitating antibodies in hypersensitivity pneumonitis. J Lab Clin Med. 1974;84:298-306.
10. California Department of Health Services, Environmental Health Investigations Branch: Misinterpretatin of Stachybotrys serology, 2000. www.dhs.ca.gov/ps/deodc/ehib/ehib2/topics/serologyf2.htm, accessed 2002.
11. Greenberger PA. Allergic bronchopulmonary aspergillosis, allergic fungal sinusitis, and hypersensitivity pneumonitis. Clin Allergy Immunol. 2002;16:449-68.
12. Greenberger PA, Patterson R. Diagnosis and management of allergic bronchopulmonary aspergillosis. Ann Allergy. 1986;56:444-8.
13. Cockrill BA, Hales CA. Allergic bronchopulmonary aspergillosis. Ann Rev Med. 1999;50:303-16.
14. Zhaoming W, Lockey RF. A review of allergic bronchopulmonary aspergillosis. J Investig Allergol Clin Immunol. 1996;6:144-51.
15. Slavin RG. Allergic bronchopulmonary aspergillosis. Clin Rev Allergy. 1985;3:167-82.
16. Katzenstein AL, Sale SR, Greenberger PA. Allergic Aspergillus sinusitis: a newly recognized form of sinusitis. J Allergy Clin Immunol. 1983;72:89-93.
17. deShazo RD, Swain RE. Diagnostic criteria for allergic fungal sinusitis. J Allergy Clin Immunol. 1995;96:24-35.
18. Schubert MS, Goetz DW. Evaluation and treatment of allergic fungal sinusitis. I. Demographics and diagnosis. J Allergy Clin Immunol. 1998;102:387-94.
19. Schubert MS. Fungal rhinosinusitis: diagnosis and therapy. Curr Allergy Asthma. Rep 2001;1:268-76.
20. Blonz ER. Is there an epidemic of chronic candidiasis in our midst? JAMA. 1986;256:3138-9.
21. Executive Committee of the American Academy of Allergy and Immunology. Clinical ecology. J Allergy Clin Immunol. 1986;78:269-71.
22. Hawkins C, Armstrong D. Fungal infections in the immunocompromised host. Clin Haematol. 1984;13:599-630.
23. Walsh TJ, Dixon DM. Nosocomial aspergillosis: environmental microbiology, hospital epidemiology, diagnosis and treatment. Eur J Epidemiol. 1989;5:131-42.
24. Singh N. Trends in the epidemiology of opportunistic fungal infections: predisposing factors and the impact of antimicrobial use practices. Clin Infect Dis. 2001;33:1692-6.
25. Munoz P, Burillo A, Bouza E. Environmental surveillance and other control measures in the prevention of nosocomial fungal infections. Clin Microbiol Infect. 2001;7 Suppl 2: 38-45.
26. Ciegler A, et al. Mycotoxins: occurrence in the environment. In: Shank RC, ed. Mycotoxins and N-nitroso Compounds: Environmental Risks. Volume I. Boca Raton, FL: CRC Press, Inc.; 1981:1-50.
27. Committee on Protection Against Mycotoxins. National Research Council. Protection against trichothecene mycotoxins. 1983. Washington, DC, National Academy Press.
28. Hendry KM, Cole EC. A review of mycotoxins in indoor air. J Toxicol Environ Health. 1993;38:183-98.
29. Nikulin M, et al. Stachybotrys atra growth and toxin production in some building materials and fodder under different relative humidities. Appl Environ Microbiol. 1994;60:3421-24.
30. Rao CY. Toxigenic fungi in the indoor environment. In: Spengler JD, Samset JM, McCarthy JS, eds. Indoor Air Quality Handbook. McGraw Hill; 2001:46-2 and 46-4.
31. Nikulin M, et al. Experimental lung mycotoxicosis in mice induced by Stachybotrys atra. Int J Exp Pathol. 1996;77:213-8.
32. Jarvis BB, et al. Study of toxin production by isolates of Stachybotrys chartarum and Memnoniella echinata isolated during a study of pulmonary hemosiderosis in infants. Appl Environ Microbiol. 1998;64:3620-5.
33. Vesper SJ, et al. Hemolysis, toxicity, and randomly amplified polymorphic DNA analysis of Stachybotrys chartarumstrains. Appl Environ Microbiol. 1999;65:3175-81.
34. Andersen B, Nielsen KF, Jarvis BB. Characterization of Stachybotrys from water-damaged buildings based on morphology, growth, and metabolic production. Mycologia. 2002;94(3):392-403.
35. Tobin RS, et al. Significance of fungi in indoor air: report of a working group. Can J Public Health. 1987;78:S1-S32.
36. Smith JE, et al. Cytotoxic fungal spores in the indoor atmosphere of the damp domestic environment. FEMS Microbiol Lett. 1992;79:337-43.
37. Rao CY, Burge HA, Chang JC. Review of quantitative standards and guidelines for fungi in indoor air. J Air Waste Manag Assoc. 1996;46:899-908.
38. Tuomi T, et al. Mycotoxins in crude building materials from water-damaged buildings. Appl Environ Microbiol. 2000;66:1899-904.
39. Schiefer HB. Mycotoxins in indoor air: a critical toxicological viewpoint. Indoor air ˆ¢90: Proceedings of the fifth international conference on indoor air. 167-72. 1990.
40. World Health Organization. Selected mycotoxins: ochratoxins, trichothecenes, ergot. Environmental Health Criteria 105. Geneva: 1990:30,77,169.
41. Drobotko VG. stachybotryotoxicosis: a new disease of horses and humans. Am Rev Soviet Med. 1945;2:238-42.
42. Kaminski E, Stawicki S, Wasowicz E. Volatile flavor compounds produced by molds of Aspergillus,. Pennicillium, and Fungi imperfecti. Appl Microbiol. 1974;27:1001-4.
43. Pohland AE. Mycotoxins in review. Food Addit Contam. 1993;10:17-28.
44. Forgacs J, Carll WT. Mycotoxicoses. Adv Vet Sci. 1962;7:273-382.
45. Ciegler A, Bennett JW. Mycotoxins and mycotoxicoses. BioScience. 1980;30:512-15.
46. Hudler GW. Magical Mushrooms, Mischievous Molds. Princeton University Press, 1998.
47. Emanuel DA, Wenzel FJ, Lawton BR. Pulmonary mycotoxicosis. Chest. 1975;67:293-7.
48. Di Paolo N, et al. Inhaled mycotoxins lead to acute renal failure. Nephrol Dial Transplant. 1994;9 Suppl 4:116-20.
49. National Institute for Occupational Safety and Health (NIOSH). Preventing organic dust toxic syndrome. 1994 Apr.
50. Pratt DS, May JJ. Feed-associated respiratory illness in farmers. Arch Environ Health. 1984;39:43-8.
51. Brinton, W. T., Vastbinder, E. E., Greene, J. W., Marx, J. J., Jr, Hutcheson, R. H., Schaffner, W.: An outbreak of organic dust toxic syndrome in a college fraternity. JAMA 1987; 258:1210-1212.
52. May JJ, et al. A study of silo unloading: the work environment and its physiologic effects. Am J Ind Med. 1986;10:318.
53. Lacey J, Crook B. Fungal and actinomycete spores as pollutants of the workplace and occupational allergens. Ann Occup Hyg. 1988;32:515-33.
54. Malmberg P, Rask-Andersen A, Rosenhall L. Exposure to microorganisms associated with allergic alveolitis and febrile reactions to mold dust in farmers. Chest. 1993;103:1202-9.
55. Croft WA, Jarvis BB, Yatawara CS. Airborne outbreak of trichothecene toxicosis. Atmospheric Environment. 1986;20:549-52.
56. Johanning E, Morey PR, Jarvis BB. Clinical-epidemiological investigation of health effects caused by Stachybotrys atra building contamination. Proceedings of Indoor Air ˆ¢93: Health effects 1993;1:225-30.
57. Johanning E, et al. Health and immunology study following exposure to toxigenic fungi (Stachybotrys chartarum ) in a water-damaged office environment. Int Arch Occup Environ Health. 1996;68:207-18.
58. Hodgson MJ, et al. Building-associated pulmonary disease from exposure to Stachybotrys chartarum and Aspergillus versicolor. JOEM. 1998;40:241-9.
59. Jarvis BB. Mycotoxins and indoor air quality. In: Morey PR, Feeley JC, Otten JA, eds. Biological Contaminants in Indoor Environments. Philadelphia: ASTM, 1990:201-14.
60. Flannigan B, Miller JD. Health implications of fungi in indoor environments: an overview. In: Samson RA, et al, eds. Health Implications of Fungi in Indoor Environments. Amsterdam: Elsevier, 1994:3-28.
61. Menzies D, Bourbeau J. Building-related illnesses. N Engl J Med. 1997;337:1524-31.
62. Fung F, Clark R, Williams S. Stachybotrys, a mycotoxin-producing fungus of increasing toxicologic importance. J Toxicol Clin Toxicol. 1998;36:79-86.
63. Robbins CA, et al. Health effects of mycotoxins in indoor air: a critical review. Appl Occup Environ Hyg.2000;15:773-84.
64. Sudakin DL. Stachybotrys chartarum: current knowledge of its role in disease. MedGenMed. 2000;E11.
65. Page EH, Trout DB. The role of Stachybotrys mycotoxins in buildings related illness. Am Ind Hyg Assoc J. 2001;62:644-8.
66. Terr AI. Stachybotrys: relevance to human disease. Ann Allergy Asthma Immunol. 2001;87:57-63.
67. Burge HA. Fungi: toxic killers or unavoidable nuisances? Ann Allergy Asthma Immunol. 2001;87:52-6.
68. Centers for Disease Control and Prevention (CDC). Acute pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, January 1993-November 1994. MMWR Morb Mortal Wkly Rep. 1994;43:881-83.
69. Centers for Disease Control and Prevention (CDC). Update: pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, Ohio, 1993-1996. MMWR Morb Mortal Wkly Rep. 1997;46:33-5.
70. Monta–a E, et al. Environmental risk factors associated with pediatric idiopathic pulmonary hemorrhage and hemosiderosis in a Cleveland community. Pediatrics. 1997;99:e5.
71. Etzel RA, et al. Acute pulmonary hemorrhage in infants associated with exposure to Stachybotrys atra and other fungi. Arch Pediatr Adolesc Med. 1998;152:757-62.
72. Centers for Disease Control and Prevention (CDC). Availability of case definition for acute idiopathic pulmonary hemorrhage in infants. MMWR Morb Mortal Wkly Rep. 2001;50:494-95.
73. Centers for Disease Control and Prevention (CDC). Update: pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, Ohio, 1993-1996. MMWR Morb Mortal Wkly Rep. 2000;49:180-84.
74. Creasia DA, et al. Acute inhalation toxicity of T-2 mycotoxin in mice. Fundam Appl Toxicol. 1987;8:230-5.
75. Creasia DA, et al. Acute inhalation toxicity of T-2 mycotoxin in the rat and guinea pig. Fundam Appl Toxicol. 1990;14:54-9.
76. Rao CY, Brain JD, Burge HA. Reduction of pulmonary toxicity of Stachybotrys chartarum spores by methanol extraction of mycotoxins. Appl Environ Microbiol. 2000;66:2817-21.
77. Rao CY, Burge HA, Brain JD. The time course of responses to intratracheally instilled toxic Stachybotrys chartarum spores in rats. Mycopathologia. 2000;149:27-34.
78. EPA Office of Research and Development. Volume I: General Factors. Exposure Factors Handbook. 1997 Aug. Washington, DC, US Environmental Protection Agency.
79. Nikulin M, et al. Effects of intranasal exposure to spores of Stachybotrys atra in mice. Fundam Appl Toxicol. 1997;35:182-8.
80. Shelton BG, et al. Profiles of airborne fungi in buildings and outdoor environments in the United States. Appl Environ Microbiol. 2002;68:1743-53.
81. Macher J. Bioaerosols: assessment and control. Cincinnati, OH: American Conference of Governmental Industrial Hygienists, 1999.
82. American Industrial Hygiene Association. Report of Microbial Growth Task Force. Fairfax, VA: AIHA Press, 2001.
83. EPA Office of Air and Radiation, Indoor Air Division. Mold remediation in schools and commercial buildings. 2001 Mar. Washington DC, US Environmental Protection Agency.
2. Horner WE, et al. Fungal allergens. Clin Microbiol Rev. 1995;8:161-79.
3. Billings CG, Howard P. Damp housing and asthma. Monaldi Arch Chest Dis. 1998;53:43-9.
4. Burr ML. Health effects of indoor molds. Rev Environ Health. 2001;16:97-103.
5. Macher J. Health effects of bioaerosols. In: Macher J, ed. Bioaerosols: assessment and control. Cincinnati, OH: American Conference of Governmental Industrial Hygienists, 1999:3-1 to -12.
6. Purokivi MK, et al. Changes in pro-inflammatory cytokines in association with exposure to moisture-damaged building microbes. Eur Respir J. 2001;18:951-8.
7. Roponen M, et al. Fungal spores as such do not cause nasal inflammation in mold exposure. Inhal Toxicol. 2002;14:541-9.
8. Fink J, Zacharisen MC. Hypersensitivity Pneumonitis. In: Middleton E, Jr. et al, eds. Allergy: Principles and Practice. St. Louis: Mosby Co.; 1998:994-1004.
9. Flaherty DK, et al. Multilaboratory comparison of three immunodiffusion methods used for the detection of precipitating antibodies in hypersensitivity pneumonitis. J Lab Clin Med. 1974;84:298-306.
10. California Department of Health Services, Environmental Health Investigations Branch: Misinterpretatin of Stachybotrys serology, 2000. www.dhs.ca.gov/ps/deodc/ehib/ehib2/topics/serologyf2.htm, accessed 2002.
11. Greenberger PA. Allergic bronchopulmonary aspergillosis, allergic fungal sinusitis, and hypersensitivity pneumonitis. Clin Allergy Immunol. 2002;16:449-68.
12. Greenberger PA, Patterson R. Diagnosis and management of allergic bronchopulmonary aspergillosis. Ann Allergy. 1986;56:444-8.
13. Cockrill BA, Hales CA. Allergic bronchopulmonary aspergillosis. Ann Rev Med. 1999;50:303-16.
14. Zhaoming W, Lockey RF. A review of allergic bronchopulmonary aspergillosis. J Investig Allergol Clin Immunol. 1996;6:144-51.
15. Slavin RG. Allergic bronchopulmonary aspergillosis. Clin Rev Allergy. 1985;3:167-82.
16. Katzenstein AL, Sale SR, Greenberger PA. Allergic Aspergillus sinusitis: a newly recognized form of sinusitis. J Allergy Clin Immunol. 1983;72:89-93.
17. deShazo RD, Swain RE. Diagnostic criteria for allergic fungal sinusitis. J Allergy Clin Immunol. 1995;96:24-35.
18. Schubert MS, Goetz DW. Evaluation and treatment of allergic fungal sinusitis. I. Demographics and diagnosis. J Allergy Clin Immunol. 1998;102:387-94.
19. Schubert MS. Fungal rhinosinusitis: diagnosis and therapy. Curr Allergy Asthma. Rep 2001;1:268-76.
20. Blonz ER. Is there an epidemic of chronic candidiasis in our midst? JAMA. 1986;256:3138-9.
21. Executive Committee of the American Academy of Allergy and Immunology. Clinical ecology. J Allergy Clin Immunol. 1986;78:269-71.
22. Hawkins C, Armstrong D. Fungal infections in the immunocompromised host. Clin Haematol. 1984;13:599-630.
23. Walsh TJ, Dixon DM. Nosocomial aspergillosis: environmental microbiology, hospital epidemiology, diagnosis and treatment. Eur J Epidemiol. 1989;5:131-42.
24. Singh N. Trends in the epidemiology of opportunistic fungal infections: predisposing factors and the impact of antimicrobial use practices. Clin Infect Dis. 2001;33:1692-6.
25. Munoz P, Burillo A, Bouza E. Environmental surveillance and other control measures in the prevention of nosocomial fungal infections. Clin Microbiol Infect. 2001;7 Suppl 2: 38-45.
26. Ciegler A, et al. Mycotoxins: occurrence in the environment. In: Shank RC, ed. Mycotoxins and N-nitroso Compounds: Environmental Risks. Volume I. Boca Raton, FL: CRC Press, Inc.; 1981:1-50.
27. Committee on Protection Against Mycotoxins. National Research Council. Protection against trichothecene mycotoxins. 1983. Washington, DC, National Academy Press.
28. Hendry KM, Cole EC. A review of mycotoxins in indoor air. J Toxicol Environ Health. 1993;38:183-98.
29. Nikulin M, et al. Stachybotrys atra growth and toxin production in some building materials and fodder under different relative humidities. Appl Environ Microbiol. 1994;60:3421-24.
30. Rao CY. Toxigenic fungi in the indoor environment. In: Spengler JD, Samset JM, McCarthy JS, eds. Indoor Air Quality Handbook. McGraw Hill; 2001:46-2 and 46-4.
31. Nikulin M, et al. Experimental lung mycotoxicosis in mice induced by Stachybotrys atra. Int J Exp Pathol. 1996;77:213-8.
32. Jarvis BB, et al. Study of toxin production by isolates of Stachybotrys chartarum and Memnoniella echinata isolated during a study of pulmonary hemosiderosis in infants. Appl Environ Microbiol. 1998;64:3620-5.
33. Vesper SJ, et al. Hemolysis, toxicity, and randomly amplified polymorphic DNA analysis of Stachybotrys chartarumstrains. Appl Environ Microbiol. 1999;65:3175-81.
34. Andersen B, Nielsen KF, Jarvis BB. Characterization of Stachybotrys from water-damaged buildings based on morphology, growth, and metabolic production. Mycologia. 2002;94(3):392-403.
35. Tobin RS, et al. Significance of fungi in indoor air: report of a working group. Can J Public Health. 1987;78:S1-S32.
36. Smith JE, et al. Cytotoxic fungal spores in the indoor atmosphere of the damp domestic environment. FEMS Microbiol Lett. 1992;79:337-43.
37. Rao CY, Burge HA, Chang JC. Review of quantitative standards and guidelines for fungi in indoor air. J Air Waste Manag Assoc. 1996;46:899-908.
38. Tuomi T, et al. Mycotoxins in crude building materials from water-damaged buildings. Appl Environ Microbiol. 2000;66:1899-904.
39. Schiefer HB. Mycotoxins in indoor air: a critical toxicological viewpoint. Indoor air ˆ¢90: Proceedings of the fifth international conference on indoor air. 167-72. 1990.
40. World Health Organization. Selected mycotoxins: ochratoxins, trichothecenes, ergot. Environmental Health Criteria 105. Geneva: 1990:30,77,169.
41. Drobotko VG. stachybotryotoxicosis: a new disease of horses and humans. Am Rev Soviet Med. 1945;2:238-42.
42. Kaminski E, Stawicki S, Wasowicz E. Volatile flavor compounds produced by molds of Aspergillus,. Pennicillium, and Fungi imperfecti. Appl Microbiol. 1974;27:1001-4.
43. Pohland AE. Mycotoxins in review. Food Addit Contam. 1993;10:17-28.
44. Forgacs J, Carll WT. Mycotoxicoses. Adv Vet Sci. 1962;7:273-382.
45. Ciegler A, Bennett JW. Mycotoxins and mycotoxicoses. BioScience. 1980;30:512-15.
46. Hudler GW. Magical Mushrooms, Mischievous Molds. Princeton University Press, 1998.
47. Emanuel DA, Wenzel FJ, Lawton BR. Pulmonary mycotoxicosis. Chest. 1975;67:293-7.
48. Di Paolo N, et al. Inhaled mycotoxins lead to acute renal failure. Nephrol Dial Transplant. 1994;9 Suppl 4:116-20.
49. National Institute for Occupational Safety and Health (NIOSH). Preventing organic dust toxic syndrome. 1994 Apr.
50. Pratt DS, May JJ. Feed-associated respiratory illness in farmers. Arch Environ Health. 1984;39:43-8.
51. Brinton, W. T., Vastbinder, E. E., Greene, J. W., Marx, J. J., Jr, Hutcheson, R. H., Schaffner, W.: An outbreak of organic dust toxic syndrome in a college fraternity. JAMA 1987; 258:1210-1212.
52. May JJ, et al. A study of silo unloading: the work environment and its physiologic effects. Am J Ind Med. 1986;10:318.
53. Lacey J, Crook B. Fungal and actinomycete spores as pollutants of the workplace and occupational allergens. Ann Occup Hyg. 1988;32:515-33.
54. Malmberg P, Rask-Andersen A, Rosenhall L. Exposure to microorganisms associated with allergic alveolitis and febrile reactions to mold dust in farmers. Chest. 1993;103:1202-9.
55. Croft WA, Jarvis BB, Yatawara CS. Airborne outbreak of trichothecene toxicosis. Atmospheric Environment. 1986;20:549-52.
56. Johanning E, Morey PR, Jarvis BB. Clinical-epidemiological investigation of health effects caused by Stachybotrys atra building contamination. Proceedings of Indoor Air ˆ¢93: Health effects 1993;1:225-30.
57. Johanning E, et al. Health and immunology study following exposure to toxigenic fungi (Stachybotrys chartarum ) in a water-damaged office environment. Int Arch Occup Environ Health. 1996;68:207-18.
58. Hodgson MJ, et al. Building-associated pulmonary disease from exposure to Stachybotrys chartarum and Aspergillus versicolor. JOEM. 1998;40:241-9.
59. Jarvis BB. Mycotoxins and indoor air quality. In: Morey PR, Feeley JC, Otten JA, eds. Biological Contaminants in Indoor Environments. Philadelphia: ASTM, 1990:201-14.
60. Flannigan B, Miller JD. Health implications of fungi in indoor environments: an overview. In: Samson RA, et al, eds. Health Implications of Fungi in Indoor Environments. Amsterdam: Elsevier, 1994:3-28.
61. Menzies D, Bourbeau J. Building-related illnesses. N Engl J Med. 1997;337:1524-31.
62. Fung F, Clark R, Williams S. Stachybotrys, a mycotoxin-producing fungus of increasing toxicologic importance. J Toxicol Clin Toxicol. 1998;36:79-86.
63. Robbins CA, et al. Health effects of mycotoxins in indoor air: a critical review. Appl Occup Environ Hyg.2000;15:773-84.
64. Sudakin DL. Stachybotrys chartarum: current knowledge of its role in disease. MedGenMed. 2000;E11.
65. Page EH, Trout DB. The role of Stachybotrys mycotoxins in buildings related illness. Am Ind Hyg Assoc J. 2001;62:644-8.
66. Terr AI. Stachybotrys: relevance to human disease. Ann Allergy Asthma Immunol. 2001;87:57-63.
67. Burge HA. Fungi: toxic killers or unavoidable nuisances? Ann Allergy Asthma Immunol. 2001;87:52-6.
68. Centers for Disease Control and Prevention (CDC). Acute pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, January 1993-November 1994. MMWR Morb Mortal Wkly Rep. 1994;43:881-83.
69. Centers for Disease Control and Prevention (CDC). Update: pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, Ohio, 1993-1996. MMWR Morb Mortal Wkly Rep. 1997;46:33-5.
70. Monta–a E, et al. Environmental risk factors associated with pediatric idiopathic pulmonary hemorrhage and hemosiderosis in a Cleveland community. Pediatrics. 1997;99:e5.
71. Etzel RA, et al. Acute pulmonary hemorrhage in infants associated with exposure to Stachybotrys atra and other fungi. Arch Pediatr Adolesc Med. 1998;152:757-62.
72. Centers for Disease Control and Prevention (CDC). Availability of case definition for acute idiopathic pulmonary hemorrhage in infants. MMWR Morb Mortal Wkly Rep. 2001;50:494-95.
73. Centers for Disease Control and Prevention (CDC). Update: pulmonary hemorrhage/hemosiderosis among infants ˆ Cleveland, Ohio, 1993-1996. MMWR Morb Mortal Wkly Rep. 2000;49:180-84.
74. Creasia DA, et al. Acute inhalation toxicity of T-2 mycotoxin in mice. Fundam Appl Toxicol. 1987;8:230-5.
75. Creasia DA, et al. Acute inhalation toxicity of T-2 mycotoxin in the rat and guinea pig. Fundam Appl Toxicol. 1990;14:54-9.
76. Rao CY, Brain JD, Burge HA. Reduction of pulmonary toxicity of Stachybotrys chartarum spores by methanol extraction of mycotoxins. Appl Environ Microbiol. 2000;66:2817-21.
77. Rao CY, Burge HA, Brain JD. The time course of responses to intratracheally instilled toxic Stachybotrys chartarum spores in rats. Mycopathologia. 2000;149:27-34.
78. EPA Office of Research and Development. Volume I: General Factors. Exposure Factors Handbook. 1997 Aug. Washington, DC, US Environmental Protection Agency.
79. Nikulin M, et al. Effects of intranasal exposure to spores of Stachybotrys atra in mice. Fundam Appl Toxicol. 1997;35:182-8.
80. Shelton BG, et al. Profiles of airborne fungi in buildings and outdoor environments in the United States. Appl Environ Microbiol. 2002;68:1743-53.
81. Macher J. Bioaerosols: assessment and control. Cincinnati, OH: American Conference of Governmental Industrial Hygienists, 1999.
82. American Industrial Hygiene Association. Report of Microbial Growth Task Force. Fairfax, VA: AIHA Press, 2001.
83. EPA Office of Air and Radiation, Indoor Air Division. Mold remediation in schools and commercial buildings. 2001 Mar. Washington DC, US Environmental Protection Agency.
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