ASHRAE IJHVAC 16-2-2010 HVAC&R Research (Volume 16 Number 2 March 2010)《《HVAC&R研究》第16卷 2号 2010年3月》.pdf
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1、Volume 16, Number 2, March 2010An International Journal of Heating, Ventilating,Air-Conditioning and Refrigerating ResearchAmerican Society of Heating, Refrigerating and Air-Conditioning Engineers, Inc.Volume 16, Number 2, March 2010HVAC accepted December 4, 2009This paper is based on findings resul
2、ting from ASHRAE Research Project RP-1243.Musty odors, often associated with damp or water-damaged buildings, originate from therelease of microbial volatile organic compounds (MVOCs) from mold growing on buildingmaterials and construction substrates. Chemical analysis of air samples is a feasible w
3、ay to sup-plement conventional bioaerosol techniques during building investigations. Analytical method-ologies for MVOCs are straightforward; however, development of a scientifically validatedmethod to measure unique MVOCs that indicate with high confidence the presence of hiddenmold regardless of t
4、he amount of mold present remains a challenge.Laboratory studies identified and quantified specific MVOCs associated with various moldspecies and MVOCs generated by specific molds growing on selected building materials in sim-ulated, realistic conditions.This research determined that numerous MVOCs
5、are released from active mold growth andare dependent on both the type of mold and the host substrate. MVOC profiles generated by 32combinations of various molds and materials were determined, but only a few of these com-pounds demonstrated effectiveness in field/building studies. Certain mold-selec
6、tive MVOCswere identified as potential indicators for specific mold, including methoxybenzene for Stachy-botrys chartarum and benzothiazole and menthol for Chaetomium globosum. These studies pro-vided a firm foundation for continued research of mold-specific MVOC markers as indicators ofhidden mold
7、and as predictors of potential mold sources in problem buildings.INTRODUCTIONIt is well known that fungal growth produces emissions as a result of secondary metabolicprocesses (Horner and Miller 2003). These microbial volatile organic compounds (MVOCs)represent a variety of chemical classes includin
8、g alcohols, amines, aldehydes, ketones, sulfides,and many other hydrocarbons (Claeson et al. 2006; Lancker et al. 2008). Therefore, in order toeffectively apply MVOC analysis to building investigations, MVOCs that are identified asmold-indicators must be unique. In other words, the MVOCs should not
9、be among the hundredsof common chemicals that emit from building materials and consumer products but should bespecific indicators of mold growth. While the literature contains studies that have been per-formed to identify MVOC emissions on building materials contaminated with mold, many ofthem do no
10、t reference the use of un-inoculated materials (negative controls); thus, it is not clearStephany Mason is technical director and W. Elliot Horner is principal consultant at Air Quality Sciences, Inc. in Mar-ietta, GA. Don Cortes is laboratory director for STAT Analysis in Chicago, IL.01_Mason.fm Pa
11、ge 109 Monday, March 1, 2010 8:49 AM 2010, American Society of Heating, Refrigerating and Air-Conditioning Engineers, Inc. (www.ashrae.org). Published in HVAC previous studies suggest that indoor emissions may be diluted tooquickly to reliably detected (Schleibinger et al. 2005; Schleibinger et al.
12、2008). Identification ofspecific target compounds may provide an opportunity to increase the sensitivity of the analyti-cal method and detect MVOCs when even a minimal amount of mold is present. Hence,extremely important and novel components of this research are the determination and validationof an
13、 MVOC sampling and analysis method.The objectives of this research were (1) to develop a database of MVOCs that are associatedwith types of mold growth found in problem building environments and that would be useful indetermining the presence of hidden mold growing in indoor environments and (2) to
14、accuratelydetermine MVOC emissions from building materials inoculated with mold and exposed undersimulated realistic environmental conditions (temperature, relative humidity, and ventilation airchange rate).METHODSFirst, to identify and quantify specific MVOCs associated with certain organisms grown
15、 ondifferent materials, selected species were grown and isolated in laboratory glass vessels forstatic studies. Following growth and incubation of the molds, air samples were obtained fromthe glass vessels using a passive volatile-organic-compound (VOC) collection technique andanalyzed using thermal
16、 desorption-gas chromatography/mass spectrometry (GC/MS). Specificemissions were identified using a mass spectrometric database of common indoor contaminantsand MVOCs. Potential marker compounds were chosen for specific mold types based on theuniqueness and levels of the identified MVOCs.Second, dyn
17、amic chamber studies were used to accurately determine MVOC emissions frombuilding materials inoculated with mold and exposed under realistic environmental conditions(temperature, relative humidity, and ventilation air change rate). Inoculated materials wereplaced into environmentally controlled cha
18、mbers operating under dynamic conditions. Chamberair was sampled using an active VOC collection technique and was analyzed using the VOCanalysis method previously described.Procurement of Mold-Contaminated Building MaterialsStatic Studies and Dynamic Chamber StudiesSix mold species, typical to water
19、-damaged buildings, were selected for use in static studies:Stachybotrys chartarum, Cladosporium sphaerospermum, Chaetomium globosum, Eurotiumamstelodami, Aspergillus versicolor (tested in duplicate), and Aspergillus sydowii. S. chartarumis widely publicized as a mold of great concern from a health
20、standpoint, and C. globosum iscommonly found in water-damaged environments. Furthermore, the two molds are often foundtogether in the environment. Based on these factors and on results from the static studies, only S.chartarum and C. globosum were used in subsequent dynamic chamber studies.Cultures
21、were freshly obtained from a commercial laboratory conducting analysis of air sam-ples on mold-colonized building samples. Isolated cultures of each organism were plated ontoappropriate growth media. S. chartarum, C. globosum, and C. sphaerospermum were cultivatedon PDA. CY20S was used for A. sydowi
22、i and E. amstelodami. A. versicolor was grown onB-malt. The inoculated plates were incubated at 25C for 5 to 7 days or until after sufficient col-onization and sporulation. Each organism was harvested and suspended in 0.01% Tween 80 with0.1% peptone (PepTween). Suspensions were vortexed for 2 min an
23、d then centrifuged for 20min at a minimum 3500 rpm. The pellet in each tube was washed twice and was suspended insterile 0.9% NaCl. The number of spores per milliliter of stock suspension was counted using a01_Mason.fm Page 110 Monday, March 1, 2010 8:49 AM 2010, American Society of Heating, Refrige
24、rating and Air-Conditioning Engineers, Inc. (www.ashrae.org). Published in HVAC thismaterial was not chosen for subsequent dynamic chamber studies. While ceiling tile is often asource of mold growth in buildings, its installation and use often is easily accessible for visualinspection of mold on eit
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