Kg. Whithear et al., STANDARDIZED METHOD OF AEROSOL CHALLENGE FOR TESTING THE EFFICACY OF MYCOPLASMA-GALLISEPTICUM VACCINES, Avian diseases, 40(3), 1996, pp. 654-660
A special chamber was constructed with the goal of controlling the pro
cess of aerosol infection of chickens with Mycoplasma gallisepticum (M
G). The virulent Australian MG field strain Ap3AS was used in each of
three experiments. The response to infection of layer-strain pullers w
as measured serologically, by the incidence and severity of gross lesi
ons in tracheas and air sacs, and by the relative numbers of MG isolat
ed from tracheas and air sacs 2 wk after challenge. In two of the expe
riments tracheal sections were assessed microscopically. Exposure to a
nebulized, undiluted broth culture of MG for 10, 20, or 30 min produc
ed uniformly severe lesions and serological responses. By contrast, re
sults were less severe and less consistent when doses of up to 10(8) c
olor-changing units (CCU) were injected directly into the abdominal ai
r sacs. Gross air sac lesions were consistently produced in almost all
pullets by exposure to an infectious aerosol containing 10(2)-10(3) C
CU/liter of air for 10 min and an air flow rate of 40 liters/min. This
can be achieved by nebulizing a 10(-3) dilution of a fresh, early sta
tionary phase culture of MG strain Ap3AS. However, under the condition
s of these experiments, this dose did not produce significant gross or
histologic lesions in the trachea.