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    by aerosolizinga5mL aliquot (1.0 × 107
    spores/mL) of a
    commercial suspension (CIP77.18, Pasteur Institute, Paris)
    into the reaction chamber as droplets in a high flow rate air
    stream using a peristaltic pump (6.4 × 107
    microorganismsMicroorganism Numeration. Direct quantitative analy-
    sis of bacteriawas achieved by epifluorescencemicroscopy
    using the “LIVE/DEAD Baclight Bacterial Viability kit”
    (Invitrogen) as appropriate viability indicator and staining
    method based on a membrane integrity test for easily
    distinguishing between live (with integrate membranes)
    and dead cells (with damaged ones), whatever their
    cultivability (5). Thus, the treatment efficiency can be
    directly derived fromthe viabilities (expressed in percents)
    at the inlet and the outlet of a photoreactor. This method
    is not suitable to viability of bacterial spores and the
    infectivity of viruses.However, since suchmicroorganisms
    do not enter a “viable but noncultivable state” (VBNC),
    their counts can be performed using classical heterotrophic
    plate count. Details can be found in a review dealing with
    numeration methods (5) and as SI S4.
    Efficiency Indicator.The efficiency of a biocidal treatment
    for disinfecting liquids or surfaces was usually described
    with the “logarithmic reduction” (LR). This indicator com-
    pared the concentrations before and after the treatment, so
    that the treatment efficiency was defined by this ratio, and
    expressed on a log10 scale for overcoming the low precision
    of biological numerations. However, this calculation could
    not be used here, since the numeration should be performed
    over the totality of the bacteria.
    Thus, the viability of the bacteria bioaerosol could be
    defined as the ratio between live bacteria and both live and
    dead bacteria in an air flow sampling. The bacteria viability
    in the inlet air corresponded to the viability of the starting
    suspension (µin), whereas the bacteria viability in the outlet
    air corresponded to the viability of the collected suspension
    (µout). The absence of any influence of both aerosolization
    and collection processes on the bacteria viability has been
    checked. The LR could be easily expressed using this
    percentage viability, and thus be replaced by the logarithmic
    reduction in viability (LRV) which considers that a virtual
    quantity ofmicroorganismsN0 entered the photoreactorwith
    a µin viability and left it with a µout one (eq 1).Results and Discussion
    Computational Fluid Dynamics (CFD) Study Applied to
    Annular Photoreactors. If annular photocatalytic reactors
    are irreplaceable for theoretical studies in the case of chemical
    applications because they enable determining the kinetic
    parameters and validating themechanismswhich can further
    be incorporated in CFD models, their efficiency for the
    removal of AMOs at high flow rates remains questionable.
    In order to illustrate that, the motion of spherical particles
    inside an annular photoreactor has been simulated using
    the “Fluent”CFDsoftware, as a function of the annular space
    and of the particle size ranging from 10 nm to 10 µm, at a
    constant flow rate of 5 m3
    /h (Figure 2). In such a configu-
    ration, the photocatalytically active contact surface cor-
    responded to the internal side of the external tube, with the
    flow passing through the inner space between both coaxial
    tubes, the inner tube being in ourmodel the external surface
    of the UV-A actinic lamp tube.
    For this computation, no reactions have been incorpo-
    rated in the model, the particles hitting the internal surface
    of the external wall being simply “trapped” on the photo-
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