DNA Mold Testing
What is
the best way to use QPCR for environmental mold testing?-Anon
There are different approaches for
using QPCR for mold testing. These include the identification of
mold species in bulk samples, the identification and quantification
of mold species collected in air sampling and, conducting an
Environmental Relative Moldiness Index (ERMI) assessment.
Bulk samples are often collected
from materials that are obviously infested (ceiling tiles, gypsum
board, carpeting, etc.) or suspected to be infested (wet ceiling
tile, carpet, wet spray-applied cellulose insulation). The
advantage of using QPCR in this instance is that one can both easily
identify and quantify major mold types present. The author has used
this to characterize and quantify the extent of mold infestation of
wet spray-applied cellulose insulation (WSACI) in a research study
that has been recently published (reprints are available upon
request)
QPCR has also been commonly used to
identify and quantify mold types collected as a result of air
sampling. Air sampling in such cases generally includes relative
low sample flow rates (~ 3-4 L/min) and extended sampling times
(several hours minimum; up to 24 hours desirable).
Air samples can be analyzed based
on sampling objectives and costs. Laboratories offer four or more
analyses panels(Mycometrics)
These may include a relatively low cost panel of four mold species (Aspergillus
versicolor, A. niger, Penicillium chrysogenium, Stachybotrys
chartarum) that are indicators of indoor mold contamination. A
second panel includes a total of 8 signature species associated with
water-damaged environments (additional species include Acremonium
strictum, Memnoniella echinata, Ulocladium botrydis and P.
brevicompactum/stolonifera). A third and somewhat more
expansive analysis panel includes a total of 15 species commonly
found indoors (these include 4 additional species of both
Aspergillus and Penicillium as well as Chaetomium
globsum. The most commonly used analyses panel includes 23
total species. This panel includes additional members of the genera
Aspergillus and Penicillium as well as Alternaria
alternata, Paecilomyces variotii, Scopulariopsi brevicaulis/fusca,
and Trichoderma harzianum.
It must be noted that the analysis
cost (from about $100-250/sample) for QPCR samples are much higher
than those for spore trap sampling ($25-60 per sample). These
analysis costs must, however, be placed into context with the
quality of the results obtained. As I have written previously, the
results of spore trap analyses reported by many laboratories do not
accurately quantify mold spores present in a sample and they cannot
accurately identify and quantify spores of the genera Aspergillus
and Penicillium some of the most important fungal species
found in indoor environments.
The bottom line is that consumers
of mold testing services usually buy an inferior product. Most
spore trap results reported by commercial laboratories cannot be
reliably interpreted. As a result, they are of little value in
determining whether an indoor air mold contamination and exposure
problem exists in a building.
To be continued
March 31, 2007
