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Previous Article | Next Article 
Journal of Clinical Microbiology, March 1998, p. 701-707, Vol. 36, No. 3
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Rapid Detection of Mycobacterium paratuberculosis in
Clinical Samples from Ruminants and in Spiked Environmental Samples
by Modified BACTEC 12B Radiometric Culture and Direct
Confirmation by IS900 PCR
R. J.
Whittington,1,*
I.
Marsh,1
M. J.
Turner,1
S.
McAllister,1
E.
Choy,1
G. J.
Eamens,1
D. J.
Marshall,2 and
S.
Ottaway2
NSW Agriculture, Elizabeth Macarthur
Agricultural Institute, Camden, New South Wales
2570,1 and
Agricultural Research and
Veterinary Centre, Orange, New South Wales
2500,2 Australia
Received 24 July 1997/Returned for modification 23 September
1997/Accepted 9 December 1997
 |
ABSTRACT |
The suitability of a radiometric culture medium consisting of
BACTEC 12B with PANTA PLUS, mycobactin J, and egg yolk was evaluated for detection of Mycobacterium paratuberculosis in feces,
mesenteric lymph nodes, and intestinal walls from cattle, sheep, and
goats. In addition, a simple method that would enable the rapid
identification of Mycobacterium paratuberculosis by
IS900 PCR in the primary cultures was sought so that
subculture to secondary egg-free radiometric medium could be avoided.
An ethanol extraction followed by differential centrifugation was used
to separate M. paratuberculosis from PCR inhibitors in the
primary culture. PCR was then undertaken with the pellet, after boiling
to lyse the mycobacteria; if this test was negative, the DNA in the
lysate was purified with guanidine thiocyanate and silica. Cultures of
feces, ilea, and mesenteric lymph nodes from cattle, sheep, and goats
known to have or suspected of having Johne's disease yielded positive
PCR results 1 to 7 weeks after inoculation. Similar results were
obtained with soil and pasture samples that had been spiked with
M. paratuberculosis. The results suggested that radiometric
culture was more sensitive than histopathology in detecting
M. paratuberculosis infection in sheep and goats and more
sensitive than culture on Herrold's egg yolk medium for the detection
of the infection in cattle. Of 259 individual PCR tests with samples
from cultures with growth indices of 
10,237 (91.5%) were positive,
with only 28 (11.8%) requiring both ethanol and silica preparation to
yield a positive result. Of the 22 negative PCR results for samples
from cultures with growth indices of 10, 18 were for samples from
cultures that had only just developed evidence of growth. PCR-positive cultures tended to remain PCR positive over successive weeks. Flexibility in the timing of the sampling for PCR is thus possible, facilitating batch processing of samples in large-scale disease control
programs for ruminants.
| |
INTRODUCTION |
Mycobacterium
paratuberculosis is the etiological agent of paratuberculosis or
Johne's disease, a granulomatous enteropathy mainly affecting
ruminants. Serious economic losses attributable to paratuberculosis are
documented in agricultural enterprises in many countries. In Australia,
a voluntary national disease control program for bovine
paratuberculosis has been implemented, while similar plans for the
goat, sheep, and alpaca industries are being advanced. Serology will be
used in each of the disease control programs to identify putative
infected herds or flocks; infection status will be confirmed by fecal
culture and/or postmortem examination of seropositive animals.
One of the factors that deters farmers from participating in a
voluntary paratuberculosis control program is the time taken by the
laboratory to confirm a diagnosis by culture. M. paratuberculosis is a slowly growing mycobacterium, requiring up
to 20 weeks to produce colonies on solid medium. Demonstration of
dependence on the iron-chelating compound mycobactin following
subculture onto medium with and without mycobactin has been used to
identify M. paratuberculosis and requires an additional
incubation of several weeks (15). Consequently, alternative
methods for culture and identification of M. paratuberculosis have been investigated. Identification is
now readily achieved by PCR amplification of the
IS900 gene, an element unique to M. paratuberculosis (7, 10).
In studies of human tuberculosis, rapid detection of M. tuberculosis has been achieved through the use of radiometric
culture systems in which a 14C-labelled substrate
(often palmitic acid) in a liquid medium is metabolized to
radiolabelled carbon dioxide that can be measured sensitively in the
gas phase above the culture (11). This method is known as
radiometric culture. Damato and Collins (6) applied radiometric culture to M. paratuberculosis and found it
to be more rapid than other cultural procedures, with growth being
detected as early as 9 days after inoculation of the medium. However,
the time required was found to be longer with samples from animals with
low-grade infections because they contained relatively few mycobacteria
compared with the numbers in samples from severely affected animals
(3). Radiometric culture was successfully combined with
IS900 PCR analysis to obtain relatively rapid confirmation of the M. paratuberculosis status of a sample
(4). The method involved inoculation of a primary
radiometric culture containing egg yolk and, after a growth index (GI)
was obtained, subculture to the same medium without egg yolk. A PCR
assay was undertaken from the secondary culture. While the results were
very encouraging, samples from only one cow and three alpacas were
tested, and the necessity for subculture to avoid the PCR inhibitors
present in the egg yolk added to the cost (A$5.50 per BACTEC vial) and
time required to obtain a diagnosis.
In Australia, there is a need for reliable culture techniques for the
strains of M. paratuberculosis that commonly infect sheep because these strains tend not to grow on conventional solid media (2). Recently, Skilbeck (12) used
radiometric culture to grow M. paratuberculosis from
tissues of sheep with Johne's disease in Victoria, Australia.
The aim of the present study was to evaluate radiometric culture as a
means of culturing M. paratuberculosis from feces,
mesenteric lymph nodes, and intestinal walls from cattle,
sheep, and goats. In addition, a simple method of enabling the specific
identification of M. paratuberculosis by
IS900 PCR in primary radiometric cultures containing egg
yolk was sought so that the delays and cost of subculture to secondary
radiometric media could be avoided.
| |
MATERIALS AND METHODS |
Collection and storage of samples.
Feces, mesenteric lymph
nodes, and intestinal tissues were collected from cattle, sheep, and
goats known to have or suspected of having Johne's disease. The status
of all animals was evaluated by histological examination of the ileum
(four sites 2 m apart), cecum (one site), proximal colon (one
site), and caudal mesenteric lymph node (one site) and/or by
serological examination by a gel diffusion precipitation test (goats
and sheep) and absorbed enzyme-linked immunosorbent assays (ELISAs)
(cattle, goats, and sheep) (13). Feces were collected from
the rectums of animals while they were on the farm or during postmortem
examination of animals that were killed immediately before sample
retrieval. Feces and tissues for culture were stored at 4°C overnight
and then, if required, at 
20 or 80°C, pending examinations.
Acid-fast-stained smears and histopathology.
Smears were
prepared from feces and scrapings of intestinal mucosa, dried in an
oven at 65°C, and stained by a Ziehl-Neelsen technique
(5). Tissues were fixed in 10% buffered neutral formalin, embedded in paraffin, sectioned at 5 µm, and stained with hematoxylin and eosin and by a Ziehl-Neelsen method (9).
Culture of M. paratuberculosis.
The double
incubation method of Whitlock and Rosenberger (16) was used
to prepare feces. Briefly, a fecal sample (2 to 5 g) was placed in
a 15-ml polypropylene tube containing a swab stick, which was used to
break up the feces in 10 to 12 ml of sterile normal saline. After
mixing, the tube was allowed to stand for 30 min at room temperature.
Five milliliters of the surface fluid was transferred to a fresh tube
containing 25 ml of 0.9% hexadecylpyridinium chloride (HPC; Sigma
Chemical Co., St. Louis, Mo.) in half-strength brain heart infusion
broth (Oxoid, Basingstoke, England), and the contents were allowed to
stand at 37°C for 24 h. After centrifugation at 900 × g for 30 min, the pellet was collected and resuspended in 1 ml of half-strength brain heart infusion broth with vancomycin (100 µg/ml), nalidixic acid (100 µg/ml), and amphotericin B (50 µg/ml)
(all reagents were from Sigma), and the mixture was incubated for 48 to
72 h at 37°C.
A lymph node or terminal ileum sample (tested separately) of
approximately 5 g was trimmed of fat and fibrous tissue, cut into
small pieces, and homogenized for 30 s in 2 ml of sterile normal
saline in a blender. After adding 25 ml of HPC, the homogenates were
left standing at room temperature for 48 to 72 h. The sediment from the base of the tube was collected.
For radiometric culture, 0.1 ml of the prepared fecal or tissue
sediment was inoculated into each culture vial. The radiometric medium
was based on those of Collins et al. (3) and Cousins et al.
(4) and consisted of Middlebrook 7H12 medium (BACTEC 12B;
Becton Dickinson, Sparks, Md.) with 200 µl of PANTA PLUS (Becton
Dickinson), 1 ml of egg yolk, 5 µg of mycobactin J (Allied Monitor
Inc., Fayette, Mo.), and 0.7 ml of water. The vials were incubated at
37°C for 8 weeks. The GI was determined weekly with an automatic ion
chamber (BACTEC 460; Johnston Laboratories, Towson, Md.).
For culture on solid medium, the prepared fecal sediment (250 µl) or
tissue sediment (50 µl) was inoculated onto each of three (feces) or
two (tissue) 35-ml screw-cap polystyrene Macartney tubes containing 10 ml of Herrold's egg yolk medium (HEYM) (1) containing 8 egg
yolks/liter, 0.4% (wt/vol) sodium pyruvate (Sigma), and 2 µg of
mycobactin J (Allied Monitor Inc.) per ml and a single tube of the same
medium without pyruvate. The tubes were incubated at 37°C for 20 weeks. Growth was determined visually at weeks 1, 2, 4, 6, 8, 9, 10, 12, 16, and 20. Identification of M. paratuberculosis was achieved by demonstration of mycobactin dependency. A colony from a
primary culture was streaked onto HEYM with and without mycobactin and
incubated for 1 month before the result was read. Mycobactin dependency
on HEYM was also undertaken for radiometric cultures in trial 3 by
using an inoculum of 50 µl after the cultures had been incubated for
10 weeks (see below).
Preparation of radiometric culture samples for PCR analysis.
BACTEC 12B medium containing egg is inhibitory to PCR assays
(4). Several simple methods for removing the egg yolk and overcoming the PCR inhibitor were investigated. These included a
variety of differential centrifugation protocols, heating followed by
differential centrifugation protocols, and alcohol treatments followed
by differential centrifugation. Only a method with alcohol subsequently
resulted in the successful amplification of IS900 from
cultures that were known to contain M. paratuberculosis
(see Results). All work was conducted in a class II biosafety cabinet by using precautions for the containment of radioactivity and the
protection of personnel.
Removal of residual inhibitors of PCR.
Lysates (45 µl)
were thawed, and DNA was purified from the entire lysate by binding to
silica in a column with 6 M guanidine thiocyanate according to the
manufacturer's instructions (Wizard PCR Preps DNA Purification System;
Promega Corporation, Madison, Wis.) and with the elution of purified
DNA in 50 µl of sterile distilled water. A volume of 5 µl of
purified DNA solution was added to each PCR mixture.
PCR.
A reaction volume of 50 µl containing 5 µl of the
DNA sample, 250 ng of each of the M. paratuberculosis
IS900 primers P90 (5'-GAAGGGTGTTCGGGGCCGTCGCTTAGG)
and P91 (5'-GGCGTTGAGGTCGATCGCCCACGTGAC) (10), 200 µM (each) the nucleotides dATP, dTTP,
dGTP, and dCTP, 66.8 mM Tris-HCl, 16.6 mM
(NH4)2SO4, 2.5 mM
MgCl2, 1.65 mg of bovine serum albumin per ml, 10 mM
-mercaptoethanol, and 2 U of Taq polymerase in buffer (10 mM Tris-HCl, 0.1 mM EDTA [pH 8.8]) was used. Amplification was
undertaken in 200-µl tubes in a 96-place thermal cycler (Corbett
Research, Sydney, Australia) with the following conditions: 1 cycle of
denaturation at 94°C for 2 min followed by 37 cycles of denaturation
at 94°C for 30 s, annealing at 62°C for 15 s, and
extension at 72°C for 1 min. Products of approximately 400 bp were
predicted, and the samples were evaluated for 400-bp products by
electrophoresis at 94 V for 45 min in 2% agarose gels stained with
ethidium bromide. The specificity of the reaction for IS900
was confirmed during optimization experiments by Southern hybridization
with an internal probe (10).
Experimental design.
A preincubation control sample was
taken immediately after inoculation of each radiometric culture vial. A
sample was again collected from the culture vial when its GI was 10;
thereafter, samples were collected from the vial at 7-day intervals for
up to 8 weeks. All samples were prepared with ethanol as described above. Samples that had GIs of 10 but a negative result in the PCR
assay were then purified with silica and retested by PCR.
Four trials were undertaken. The first trial was with frozen-stored
samples from cattle and sheep that were known to contain M. paratuberculosis on the basis of the results of conventional culture on solid medium (cattle) or histopathology and examination of
tissue or fecal smears stained with Ziehl-Neelsen stain (sheep). In the
second trial, samples from goats and sheep with unknown infection
status were selected for culture on the basis of the results of
serological testing, to mimic the approach taken in a disease control
program; the animals were known to have been exposed to M. paratuberculosis on a farm where Johne's disease is endemic, and
the samples were processed for culture after overnight storage at
4°C. In the third trial, feces from seropositive cattle from a herd
known to be infected were cultured to mimic the approach taken in a
disease control program. In the fourth trial, the suitability of the
culture method for environmental samples was evaluated, with the main
considerations being sensitivity, contamination with rapidly growing
environmental organisms, and inhibition of the PCR. Feces from two
sheep excreting either high or low numbers of M. paratuberculosis were mixed with soil and pasture samples to
achieve 3 log10 dilutions and were then cultured.
| |
RESULTS |
Sample preparation and purification methods.
The ethanol
extraction method described below was a simple procedure. Briefly, the
rubber stopper lid of the radiometric culture vial was wetted with 70%
ethanol, left for 20 s, and then dried. The vial was inverted
several times to mix the contents, and 200 µl of medium was removed
with a sterile syringe and needle and transferred to a screw-cap 1.5-ml
polypropylene microcentrifuge tube. Five hundred microliters of
absolute ethanol was added, and the tube was left to stand for 2 min
before mixing vigorously on a vortex mixer for 5 s and
centrifuging at 8 × g for 10 min at 22°C. Partially
flocculated egg yolk accumulated at the base and sides of the tube. The
supernatant was transferred to a clean microcentrifuge tube, and the
tube was then centrifuged at 18,000 × g for 5 min. The
resulting pellet was washed twice in 200 µl of sterile
phosphate-buffered saline by resuspension and centrifugation and was
then resuspended in 50 µl of sterile distilled water. The tube was
placed in a dry-heating block at 100°C for 20 min to lyse the
mycobacteria. A volume of 5 µl of the lysate was added to each PCR
mixture. The lysate was then stored at 20°C.
To evaluate the samples for the presence of residual inhibitors of PCR
and excess target DNA, five lysates from samples that had GIs of 10
but negative PCR results and one PCR-positive lysate were diluted 10- and 100-fold and retested by PCR, with negative results. DNA was then
purified from the same lysates with silica, diluted 10- and 100-fold,
and tested by PCR. Four samples that were previously PCR negative then
gave positive PCR results. Dilution of the purified DNA samples was
detrimental, with the PCR results then being negative.
To test whether there were significant losses of target DNA during
silica purification, three PCR-positive lysates with graded responses
were tested again to ensure the consistency of the response and were
then purified with silica and tested again. They remained PCR positive.
The intensity of the PCR product from a strongly positive sample was
slightly diminished by the silica purification. The intensities of the
PCR products from a moderately positive sample and a weakly positive
sample were enhanced, while a sample that had appeared initially
negative gave a detectable product after silica purification (Fig.
1). These results correlated with the GI.
Unless treated with ethanol, all samples were inhibitory to the PCR
assay (Fig. 1).
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FIG. 1.
Effect of sample treatment on the results of PCR
analysis. The PCR product (20 µl) was resolved on a 2% agarose gel
for 45 min at 94 V and was stained with ethidium bromide. The following
samples were tested: A, GI of 999, lanes 1 to 4; B, GI of 91, lanes 5 to 8; C, GI of 39, lanes 9 to 12; D, GI of 7, lanes 13 to 16. The
treatments were as follows: nil, lanes 1, 5, 9, and 13; ethanol, first
test, lanes 2, 6, 10, and 14; ethanol, second test, lanes 3, 7, 11, and
15; ethanol plus silica, lanes 4, 8, 12, and 16. Lane 18, DNA size
markers; lane 19, positive control with IS900; lane 20, negative control.
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Trial 1.
In the first trial, ovine and bovine samples that
were known to contain M. paratuberculosis were used.
M. paratuberculosis was cultured in radiometric medium
and was identified by IS900 PCR from each sample within 6 weeks of inoculation (Table 1). Tissues
(ileum or lymph node) yielded positive results in 1 to 4 weeks, while
feces yielded positive results in 2 to 6 weeks. When a GI of 10 was
first noted in the cultures, 5 of 12 samples prepared with ethanol
alone yielded positive PCR results. These cultures had GIs in the range
of 236 to 999. Three cultures that had lower GIs (range, 10 to 23), and
the M. paratuberculosis control culture (GI, 26)
required ethanol and silica preparation in order to yield a positive
PCR result on the first occasion that it was tested. Samples from three
of the remaining four cultures (GIs, 29, 99, 157, and 755) were PCR
negative when they were first tested, regardless of the method of
sample preparation, but they were positive 1 week later. Samples from
three cultures were PCR positive immediately after inoculation (Table
1, animals 4, 5, and 8), indicating the presence of large numbers of
M. paratuberculosis cells in the inoculum, but a GI was
not detected for 3 weeks in one of these cultures, suggesting the
presence of few viable M. paratuberculosis cells in the
original inoculum. Samples from the majority of cultures were PCR
negative immediately after inoculation, confirming that replication of
M. paratuberculosis had occurred in the medium; this
was a significant finding for the samples from sheep. In each of the
weeks following the first confirmation of growth by PCR, samples from
each of the cultures, except one in 1 week, were PCR positive after
ethanol preparation alone. The GIs of these samples ranged from 329 to
999. Overall, 80 of 85 samples examined by PCR between 1 and 8 weeks
after inoculation of the culture medium were positive; 5 of the 80 positive samples had required preparation with ethanol and silica. None
of the samples from sheep produced visible growth on HEYM after 20 weeks, while each of the bovine samples yielded colonies visible at 10 weeks.
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TABLE 1.
Culture of ovine and bovine clinical samples known to
contain M. paratuberculosis by using radiometric
medium, HEYM, and identification of M. paratuberculosis by IS900 PCR with a sample from the
primary culturea
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Trial 2.
In the second trial, samples were taken from goats
and sheep from a property on which livestock were known to have
Johne's disease. The animals were chosen on the basis of a reaction in a gel diffusion precipitation assay or absorbed ELISA for antibodies against M. paratuberculosis. A mesenteric lymph node
and feces from each animal were cultured. Four of 5 goats and 4 of 11 sheep were found by radiometric culture followed by PCR to be infected with M. paratuberculosis (Table
2). Seven lymph node samples and six
fecal samples were culture positive. Of these 13 culture-positive samples, 8 were PCR positive when a GI was first detected (GI range, 10 to 480) following ethanol preparation alone, and an additional 2 samples (GIs, 28 and 35) were PCR positive at this time after ethanol
and silica preparation. The remaining three samples were PCR negative
when a GI was first detected (GIs, 15, 107, and 207), despite ethanol
and silica preparation, but were PCR positive a week later (GI range,
586 to 999) after ethanol preparation alone (Table 2). After first
becoming PCR positive, samples collected weekly from all but one
culture in 1 week remained PCR positive for the duration of the 8-week
incubation. Two cultures were PCR positive immediately after
inoculation. Overall, 63 of 67 samples examined by PCR between 1 and 8 weeks after inoculation of the radiometric medium were positive; 2 of
the 63 positive samples had required preparation with ethanol and
silica. M. paratuberculosis was not recovered from any
of the samples cultured on HEYM during an incubation of 20 weeks.
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TABLE 2.
Culture of caprine and ovine clinical samples with
radiometric medium and identification of M. paratuberculosisa by IS900 PCR
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Culture detected a greater number of infected goats and sheep than did
the other tests. Only two of the four infected goats and three of the
four infected sheep were shown to be infected with M. paratuberculosis by examination of fecal or tissue smears stained
with Ziehl-Neelsen stain and/or histopathological examination of
the ileum, cecum, colon, and mediastinal lymph node (Table 2).
Trial 3.
In a third trial, fecal samples were cultured from 21 cows that were suspected of being infected with M. paratuberculosis on the basis of the results of serological tests,
as is done during routine surveillance for Johne's disease. Twelve
cultures were PCR positive within 7 weeks (Table
3). Of these, five were positive when
first tested (GIs, 38, 57, 460, 638, and 835), with the two with the
highest GIs requiring ethanol and silica preparation, while 7 were
negative (GI range, 11 to 121) even after silica purification. Samples
from the latter cultures were all PCR positive 1 week later (GIs, 472 to 999). Samples from two cultures were PCR negative in week 8, even
though samples from these cultures were PCR positive over the previous
2 to 4 weeks. None of the samples were PCR positive immediately after
inoculation. Overall, 50 of 59 samples examined by PCR between 1 and 8 weeks after inoculation were positive. Of the 50 positive samples, 18 had required ethanol and silica preparation. Of the 27 samples tested
by PCR after ethanol and silica preparation because of an earlier
negative PCR result, 18 were positive. M. paratuberculosis was recovered on HEYM from 8 of the 12 samples
that were culture positive in radiometric medium (Table 3). A
mycobactin dependency test on HEYM was used to identify M. paratuberculosis in the 12 PCR-positive radiometric cultures, but
the results for 3 of the 12 cultures could not be confirmed with this
method because of overgrowth of fast-growing bacterial species (Table
3).
Trial 4.
In the fourth trial, an ovine fecal sample in which
large numbers of acid-fast rods were visualized and a second ovine
fecal sample in which very small numbers of acid-fast rods were
visualized were diluted and thoroughly mixed with soil or grass
clippings so as to achieve dilutions of the feces of 1:10, 1:100, and
1:1,000. The resulting specimens were treated as described above for
fecal samples. Samples from each of the cultures were PCR positive
after 2 to 6 weeks of incubation in the radiometric medium, and
observations were discontinued at 6 weeks (Table
4). Samples from four cultures were PCR
negative on the first occasion that a GI was noted (GI range, 24 to
242) but were PCR positive a week later. Samples collected from two
cultures in week 6 required ethanol and silica preparation in order to
yield a positive PCR result. Overall, 44 of 48 samples examined by PCR
between 1 and 6 weeks after inoculation were positive; 3 of the 44 positive samples had required both ethanol and silica preparation. None
of the cultures was discarded because of contamination.
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TABLE 4.
Radiometric culture of soil and pasture samples
inoculated with ovine feces
containing M. paratuberculosisa
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In each of the trials, the GIs of the cultures increased rapidly after
becoming detectable so that 1 to 2 weeks later most had GIs equal to or
greater than the maximum level (GI, 999). Toward the end of the
incubation period, the GIs of some of the cultures declined, presumably
in association with repeated removal of the gas phase and depletion of
the labelled substrate in the liquid phase (8).
| |
DISCUSSION |
This study, like several others (3, 4), has confirmed a
useful role for radiometric culture in the detection of M. paratuberculosis, with the principal advantage over conventional
culture on solid medium being the relatively short time required before
being able to report a result. This is particularly so if PCR
amplification of the IS900 gene rather than demonstration of
mycobactin dependency is used to confirm the identities of isolates.
However, a disadvantage of this approach has been the need to
subculture samples from the primary radiometric culture vial to
radiometric medium without egg yolk in order to obtain a sample that is
noninhibitory for the PCR assay (4). The need for subculture
of samples into a secondary radiometric culture vial adds greatly to
the costs of labor and materials associated with the detection of
M. paratuberculosis. To gain a saving in time but to
avoid additional costs associated with the identification of
M. paratuberculosis by PCR after subculture, we have
routinely used primary radiometric culture and then subcultured samples
onto HEYM to demonstrate mycobactin dependency. This approach has not
been possible for ovine samples, which have generally failed to grow on
HEYM. The method that we report here enables culture in
radiometric medium followed by PCR with samples from the primary
culture for confirmation of the presence of M. paratuberculosis. In addition to savings in labor and materials,
there is a further saving in time because a second incubation period is
avoided. Our results indicated that simple treatment of samples removed from primary radiometric cultures effectively removed substances that
are inhibitory to PCR and permitted testing for the presence of the
M. paratuberculosis-specific IS900 gene.
During this study 259 individual samples from cultures obtained between
1 and 8 weeks after inoculation were examined by PCR following ethanol
or ethanol plus silica preparation, and 237 (91.5%) were positive. Of
the 22 PCR-negative samples, 18 were taken on the first occasion that a
GI was noted, 17 had GIs of <250, and 11 had GIs of <100. All these
cultures were PCR positive 1 week later, which strongly suggests that
there were insufficient M. paratuberculosis cells in
the cultures when they were first sampled. The reasons why some
cultures with relatively high GIs were PCR negative are unclear but may
include the presence of residual inhibitors of the PCR in the sample
after the treatment steps the presence in the culture of organisms
other than M. paratuberculosis which contributed to the
GI, clumped growth which resulted in the failure to include sufficient
numbers of M. paratuberculosis cells in the sample for
PCR, and excessive numbers of M. paratuberculosis or
other cells which resulted in an excess of target DNA or irrelevant DNA
in the PCR. The last possibility seems remote given the fact that
dilution of the sample for PCR failed to result in a positive result.
The chance of residual PCR inhibition is real and perhaps is overcome
only when the amount of target DNA reaches a certain level. Because
inhibitors may be contributed by the inoculum as well as the culture
medium, it is likely that the level of residual inhibition will vary
from sample to sample. There was evidence of this in the present study,
in which in trial 3 a relatively high proportion (36%) of the
PCR-positive samples required silica purification. However, overall
only 28 of 237 (11.8%) PCR-positive samples in this study required
silica purification.
General recommendations can be made regarding the timing of the PCR
examination of radiometric cultures that have evidence of growth. We
did not seek to determine the threshold GI required to yield a positive
result in PCR assays because GIs tend to increase rapidly and we wished
to monitor cultures only weekly. However, because of the factors
mentioned above that might result in negative PCR results even with
high GIs, positive PCR results probably should not be expected to be
related to a narrow threshold. This is illustrated in the present
study, in which most of the negative PCR results were in samples from
cultures with GIs of <250 but in which 17 of the 50 PCR-positive
cultures were detected when the GI was <200. For routine batch
processing of diagnostic samples it would be appropriate to wait 1 to 2 weeks after first recording a GI of >10 before undertaking PCR
examination or to undertake PCR examination of all cultures with GIs of
>200 at 6 to 8 weeks after inoculation. By either of these approaches,
most samples would be expected to yield a positive PCR result after
ethanol preparation alone. If it is desired that results be reported
after a minimum incubation period, samples from cultures with GIs
should be purified with silica before PCR examination, and if negative, a sample should be taken and tested by PCR after a further 7 days of
incubation. Certain batches of clinical samples may be troublesome and
may require the additional silica purification, but rather than doing
this routinely, it would be easier and cheaper to apply silica
purification only to those samples that gave a negative PCR result in
the first instance.
An unexpected finding from this study was that BACTEC 12B medium
containing egg yolk, mycobactin J, and PANTA PLUS appeared to be
satisfactory for culture of M. paratuberculosis strains from sheep. In Australia, these ovine strains have proven to be very
difficult to culture on conventional solid or liquid media and have
been regarded as noncultivable for practical diagnostic purposes.
Although it has been recognized since 1996 that culture of these
strains from tissues may be possible in BACTEC 12B medium (12), an inference from the unpublished findings was that
positive PCR results for samples from BACTEC 12B cultures may have been due simply to the continued presence of M. paratuberculosis organisms that were in the inoculum. We have
shown this inference to be incorrect. Replication of M. paratuberculosis determined by a change in the PCR status of the
culture from negative to positive was shown to have occurred in most
instances. Primary culture of Australian ovine strains of M. paratuberculosis on solid medium or successful subculture from
radiometric medium to solid medium has not yet been achieved reliably.
Furthermore, repeated subculture of these strains in the same
radiometric medium results in the loss of viability (unpublished
observations). Therefore, an effort is required to elucidate the
cultural requirements of M. paratuberculosis strains
from sheep in Australia.
The results of this study support and extend those of Cousins et
al. (4) and suggest that culture of clinical samples in BACTEC 12B medium with egg yolk, mycobactin J, and PANTA
PLUS can enable the relatively rapid detection of the principal types of M. paratuberculosis that are endemic in Australia.
Johne's disease is known to occur in cattle, goats, sheep, and alpacas in Australia and is associated with infection with several distinct genotypes of M. paratuberculosis. Although we did not
include samples from infected alpacas, isolates of M. paratuberculosis from alpacas have been found to be similar to
isolates from cattle and can be grown in modified BACTEC 12B medium
(4).
The fact that several culture-positive sheep and goats were classified
as uninfected on the basis of histopathology and examination of fecal
or tissue smears suggests that radiometric culture followed by
IS900 PCR may be more sensitive than the other tests and may be able to detect relatively few bacteria in tissue or fecal samples. It is reasonable to speculate on the numbers of M. paratuberculosis cells that might have been present in the spiked
soil and pasture samples used in this study. On the basis of a likely
detection limit of 103 to 104 organisms per
gram by microscopic examination of smears stained with Ziehl-Neelsen
stain (14), the soil and pasture samples prepared with the
highest final dilution of feces with low numbers of organisms (Table 4)
would have contained 1 to 10 to 10 to 100 cells per g. Unfortunately,
we were unable to obtain samples from cattle with very low numbers of
M. paratuberculosis organisms in their tissues or
feces, as was a problem in a previous study (4).
Consequently, we are still unsure of the sensitivity of radiometric
culture compared to that of conventional culture on solid medium for
the detection of animals in the early stages of infection with strains
of M. paratuberculosis that can be grown on solid
media. For this reason we plan to compare radiometric culture and
conventional culture over a longer period to establish the relative
sensitivities of these methods. However, the preliminary results (Table
3) suggest that radiometric culture may be more sensitive than culture
on HEYM.
The radiometric culture and PCR preparation methods described here
appeared to be suitable for culture and identification of M. paratuberculosis from soil and pasture samples that had been
spiked with the organism. There did not appear to be contamination of
cultures with rapidly growing environmental actinomycetes and fungi,
and PCR inhibition appeared to be minimal.
Radiometric cultures are incubated for only 8 weeks before a negative
result is reported, whereas conventional cultures require 20 weeks of
incubation on solid medium. M. paratuberculosis was detected within 7 weeks in all culture-positive samples evaluated in
this study. The time saved through the use of radiometric culture followed directly by IS900 PCR may remove a significant
impediment to the adoption of disease control programs for Johne's
disease in ruminants. These programs are based on herd screening by
serology, which may yield some seropositive individuals that must be
examined by culture. Farmers are sometimes reluctant to enter into a
program that creates uncertainty about infection status when
clarification of infection status cannot be made for 5 to 6 months.
Radiometric culture with the identification of M. paratuberculosis by IS900 PCR offers a 3- to 4-month
respite from this uncertainty.
| |
ACKNOWLEDGMENTS |
We gratefully acknowledge the financial assistance of the
McGarvie Smith Trust, without which this study would not have been possible.
Andrew Berneutz provided valuable technical assistance in the early
stages of this study.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: NSW Agriculture,
Elizabeth Macarthur Agricultural Institute, PMB 8, Camden, NSW 2570, Australia. Phone: 61 293343. Fax: 61 293384. E-mail:
whittir{at}agric.nsw.gov.au.
| |
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Abstract
Introduction
