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Applied and Environmental Microbiology, September 1998, p. 3153-3158, Vol. 64, No. 9
Department of Food Science (Food
Microbiology),
Received 3 November 1997/Accepted 10 June 1998
An immunomagnetic separation (IMS) technique was developed to
facilitate selective isolation of Mycobacterium
paratuberculosis cells from milk. Rabbit polyclonal antibodies
against radiation-killed intact M. paratuberculosis
cells were produced and used to coat sheep anti-rabbit immunoglobulin G
(IgG) type M-280 Dynabeads. The rabbit anti-M.
paratuberculosis IgG-coated beads (IMB) reacted strongly with
laboratory strains of M. paratuberculosis as
determined by slide agglutination, and microscopic examination
confirmed that M. paratuberculosis cells attached to
the IMB. The IMB were found to have a maximum binding capacity of
104 to 105 CFU of M. paratuberculosis. Studies showed that IMS selectively recovered
M. paratuberculosis from inoculated milk containing as
few as 10 CFU of M. paratuberculosis per ml when 10 µl of IMB (ca. 106 beads) was added to 1 ml of milk and
the preparation was incubated for 30 min at room temperature with
gentle agitation. Larger volumes of milk (10 and 50 ml) were
centrifuged and resuspended in 1 ml of phosphate-buffered
saline-0.05% Tween 20 prior to IMS in order to increase the
sensitivity of the method. Currently, primary isolation of
M. paratuberculosis from a milk sample relies on chemical decontamination, followed by culturing on Herrold's egg yolk
medium, which must be incubated at 37°C for up to 18 weeks. The
potential value of our IMS method is as an aid for rapid detection of
M. paratuberculosis in milk when it is used in
conjunction with end point detection methods, such as IS900
PCR or an enzyme-linked immunosorbent assay.
Mycobacterium
paratuberculosis causes paratuberculosis, commonly known
as Johne's disease, in cattle, sheep, goats, and other ruminants
(2). Although not currently classified as a zoonotic agent,
M. paratuberculosis has been identified in intestinal
biopsy tissues from some patients with Crohn's disease (CD)
(1). CD is a chronic, incurable, low-grade inflammation of
the terminal ileum, one of two similar diseases of the human
gastrointestinal tract known as inflammatory bowel disease. Whether the
presence of M. paratuberculosis in biopsy material
indicates that this organism has a causative role in CD or is simply a
complicating infection is still the subject of much debate. However, if
M. paratuberculosis has a causative role in CD, then
milk may be a possible vehicle of transmission of the organism from
cattle to humans (7, 21). Detectable quantities of
M. paratuberculosis have previously been found in the
milk of both clinically infected (20) and subclinically
infected (18, 19) cattle with Johne's disease. One theory
put forward to explain the increasing incidence of CD in humans in
certain parts of the world is that the human population may be
repeatedly exposed to low levels of M. paratuberculosis in the milk supply (7). This explains the interest in
determining whether M. paratuberculosis is present
in the general supply of fluid milk, both raw and pasteurized. Only one
such study has been published to date. Millar et al. (13)
used IS900 PCR to detect M. paratuberculosis
in retail pasteurized cow's milk in England and Wales and reported
that overall, 7% of 312 milk samples tested positive for the presence
of M. paratuberculosis DNA over a 19-month period. At
peak periods up to 25% of the milk samples were positive as determined
by IS900 PCR. However, the presence of viable cells was
never confirmed by decontamination and culturing of PCR-positive milk
samples, so the theory of repeated exposure of humans to viable
M. paratuberculosis in milk was not substantiated by
the results of this milk survey.
Determination of the incidence of M. paratuberculosis
in milk supplies is fraught with difficulties. First, M. paratuberculosis is an extremely slow-growing organism which can
take up to 20 weeks for primary isolation, whereas most other
microorganisms in milk exhibit growth within 24 to 48 h. As
no selective medium for M. paratuberculosis is
available, successful isolation of M. paratuberculosis
currently relies on selective suppression of nonmycobacterial
contaminants in samples by chemical decontamination. The recommended
decontamination procedure for M. paratuberculosis is
treatment with 0.75% (final concentration) hexadecylpyridinium chloride (HPC) for several hours (23). A balance must be
struck between adequate time for decontamination and the possibility of
undue damage to the M. paratuberculosis cells if the
decontamination period is too long. Unless adequate decontamination is
achieved, any surviving undesirable microorganisms quickly overgrow the M. paratuberculosis colonies, thwarting isolation
efforts. All of the milk surveys carried out to date (13,
18-20) have relied on chemical decontamination in some shape or
form prior to culturing of M. paratuberculosis from
milk. Second, M. paratuberculosis is likely to be
present in low numbers in naturally infected milk samples. A titer of
just 2 to 8 CFU of M. paratuberculosis per 50 ml of
milk has been reported for milk obtained aseptically from asymptomatic
cattle with Johne's disease (19). Consequently, the culture
methods employed to isolate M. paratuberculosis must be
extremely sensitive, or, alternatively, the sensitivity of the culture method employed must be improved by concentrating the
M. paratuberculosis cells prior to culturing. In
theory, immunomagnetic separation (IMS) could be used to resolve
these difficulties.
IMS is a simple but powerful method for extracting a desired organism
from heterogeneous bacterial suspensions, such as those that are
encountered in food, clinical specimens, and feces (3, 15). It has previously been used successfully with several types of food samples, including milk (8, 14, 16, 17). IMS relies
on the interaction between cell surface antigens and antibodies attached to paramagnetic beads. The desired cells are separated by
placing a bead suspension in a strong magnetic field. The beads can be
resuspended after IMS in a smaller volume of liquid, thereby concentrating the sample. If appropriate antibodies directed against surface antigens of M. paratuberculosis were obtained
or produced, this organism could be selectively isolated from milk
samples and concentrated by IMS, thereby improving the specificity and sensitivity of subsequent culture methods. During IMS the M. paratuberculosis cells would not be exposed to potentially
damaging chemicals, as they are during traditional
decontamination procedures, and, consequently, the physiological
state of the cells would not be affected. Previous applications of IMS
in mycobacteriology include detection of Mycobacterium avium
in stool samples from AIDS patients (10) and detection of
Mycobacterium tuberculosis in cerebrospinal fluid
(11).
In this paper we describe the development, optimization, and evaluation
of an IMS procedure to facilitate the isolation of M. paratuberculosis from milk samples.
Production of rabbit anti-M. paratuberculosis
antiserum.
Colonies of M. paratuberculosis B4 (a
bovine field strain isolated in Northern Ireland) grown on Herrold's
egg yolk medium (HEYM) were suspended in phosphate-buffered saline
(PBS), and the preparation was centrifuged, washed five times in PBS,
and then irradiated (dose, 15 kGy) with a Gammabeam 650 instrument (Nordion International Inc., Kanata, Ontario, Canada) in order to kill
the cells. A 0.5-ml portion of a dense suspension (concentration, approximately 108 CFU/ml) of irradiated cells was mixed
with an equal volume of the adjuvant Quil A (125 µg per ml; Superfos,
Vedbaek, Denmark) and used to inoculate a rabbit subcutaneously at
multiple sites. This inoculation procedure was repeated after 5 weeks,
followed (at 15- to 20-day intervals) by three intravenous inoculations of 0.5 ml. The rabbit was test bled 7 to 14 days after the second subcutaneous inoculation and after each intravenous inoculation. The
antiserum obtained was tested by an enzyme-linked immunosorbent assay
(ELISA) in which microtiter wells were coated with the cell suspension
used to inoculate the rabbit; HEYM was used as a control. No ELISA
reaction was obtained with the HEYM antigen. The rabbit was
exsanguinated 14 days after a titer greater than 1:3,000 was recorded
with the M. paratuberculosis antigen; the serum was
separated and stored at Purification of the polyclonal rabbit anti-M.
paratuberculosis serum.
The rabbit anti-M.
paratuberculosis serum was purified by precipitating albumin and
other non-immunoglobulin G (IgG) proteins with caprylic acid (25 µg
per ml) after 2 volumes of 0.06 M acetate buffer (pH 4.3) was added by
the method of McKinney and Parkinson (12). After
centrifugation at 10,000 × g for 15 min, the
precipitate was discarded, and the IgG fraction was dialyzed overnight
at 4 to 10°C against 0.01 M PBS (pH 7.2). The purified polyclonal IgG
was divided into 1-ml aliquots and stored at Specificity of the polyclonal rabbit anti-M.
paratuberculosis IgG.
Slide agglutination was used to test
for cross-reactions of the polyclonal IgG with other
Mycobacterium spp. and bacterial isolates obtained from raw
milk. Twenty microliters of undiluted polyclonal IgG was applied to a
clean slide. A loopful of the test organism was mixed with the IgG, the
slide was tilted several times, and agglutination was checked within 2 min. The slide agglutination test was repeated by using 20-µl
portions of 1:10, 1:100, and 1:1,000 dilutions of the polyclonal IgG in
PBS.
Coating of magnetic beads.
The polyclonal IgG was used to
coat sheep anti-rabbit IgG type M-280 Dynabeads (catalog no. 11203;
Dynal UK Ltd., Wirral, United Kingdom) for 24 h at 2 to 4°C as
recommended by the manufacturer. In all of the IMS trials 10-µl
aliquots (ca. 106 beads) of the rabbit anti-M.
paratuberculosis IgG-coated beads (IMB) were employed.
Strains studied.
Three M. paratuberculosis
strains were used in this study. These strains were type strain NCTC
8578 and field strains B2 and B4, which were previously isolated from
cattle in Northern Ireland. The culture conditions used and the method
used to prepare the inoculum have been described previously
(6). In addition, Mycobacterium intracellulare
NCTC 10425, Mycobacterium kansasii NCTC 10268, and a field
strain of M. avium were used to test the
specificity of the polyclonal IgG.
Milk samples.
Milk samples with low levels of background
microflora (either raw cow's milk aseptically obtained from a healthy
Friesian cow as described previously [6] or
pasteurized whole cow's milk routinely sent to the Food Microbiology
Unit for testing), were used in this study.
Confirmation of M. paratuberculosis attachment
to IMB.
In order to visualize M. paratuberculosis
cells bound to the IMB after IMS, 2 drops of a bead-cell suspension was
transferred to a microscope slide, air dried, and then heat fixed. The
smear was flooded with a 0.1% (wt/vol) phenolic auramine O solution for 15 min, decolorized with acid-alcohol for 2 min, counterstained with a 0.3% (wt/vol) methylene blue solution for 2 min, and then allowed to air dry prior to microscopic examination under blue light
(9). Acid-fast cells fluoresced bright yellow against a dark
background, whereas the IMB fluoresced only weakly.
Determination of the optimum immunocapture time and percentage of
recovery.
Seven 1-ml aliquots of milk and three 1-ml aliquots of
PBS were each inoculated with 106 CFU of M. paratuberculosis NCTC 8578. One of the inoculated milk samples was
immediately serially diluted and cultured on HEYM slopes in order to
determine the number of M. paratuberculosis cells added
to the samples prior to IMS. Another three inoculated milk samples were
centrifuged (2,500 × g for 15 min) and resuspended in
1 ml of PBS before IMS; these samples were designated milk/PBS samples.
Ten microliters of coated Dynabeads was added to each inoculated sample
(three milk samples, three milk/PBS samples, and three PBS samples),
and the tubes were incubated on a Dynal sample mixer at room
temperature (21°C) for 15, 30, or 60 min. After a 15-min
immunocapture, one milk sample, one milk/PBS sample, and one PBS sample
were removed and processed by using the remainder of the IMS procedure.
Following IMS, the IMB were resuspended in 1 ml of PBS. After 30- and
60-min immunocapture times, three additional tubes were removed and
processed in the same way. All samples were then diluted as necessary,
and the number of M. paratuberculosis cells recovered
by IMS from each of the suspending media after each of the
immunocapture times was determined by culturing on HEYM slopes. The
percentage of recovery of M. paratuberculosis cells
from each milk or PBS sample was calculated on the basis of the number
of cells which attached to the IMB. The same experiment was performed
with M. paratuberculosis B2.
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Isolation of Mycobacterium
paratuberculosis from Milk by Immunomagnetic
Separation
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
20°C.
20°C.
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FIG. 1.
Schematic diagram of the optimized IMS procedure for
detection of M. paratuberculosis in milk. N, magnet.
Use of centrifugation prior to IMS to concentrate M. paratuberculosis cells. Different volumes of raw milk (5, 10, and 50 ml) were inoculated with a fixed number of M. paratuberculosis cells (approximately 106 CFU). Each milk sample was centrifuged at 2,500 × g for 15 min, and the pellet was resuspended in 1 ml of PBS-T prior to IMS. Following IMS, the IMB were resuspended in 1 ml of sterile water, and the number of M. paratuberculosis cells recovered from each milk sample volume was determined by serial dilution and inoculation of HEYM slopes (100 µl per slope). Colony counts were obtained after incubation of the slopes for up to 12 weeks at 37°C. This experiment was repeated twice.
In order to assess whether the majority of the M. paratuberculosis cells present in a milk sample were located in the pellet after centrifugation, two 10-ml samples of raw milk were inoculated with a fixed number of M. paratuberculosis cells (approximately 106 CFU) and centrifuged at 2,500 × g for 15 min in order to obtain the following three milk fractions: cream, whey, and pellet. The cream and pellet fractions were resuspended in 1 ml of PBS to facilitate enumeration of the M. paratuberculosis cells present. The whey fraction was tested directly. Following dilution as necessary, the number of M. paratuberculosis cells in each fraction was determined by inoculating HEYM slopes (100 µl per slope) and counting the colonies after incubation for up to 12 weeks at 37°C. The percentage of M. paratuberculosis cells in each fraction was calculated by taking into account the dilution of the cream and pellet layers and the volume of each milk fraction.Determination of the minimum detection limit of the IMS method. An inoculated milk sample containing 108 CFU of M. paratuberculosis/ml (the size of the inoculum was confirmed by dilution and plating on HEYM) was serially diluted in milk to obtain a set of eight milk samples containing between 101 and 108 CFU of M. paratuberculosis/ml. A 1-ml aliquot of each of the milk samples was then subjected to IMS and resuspended in 1 ml of PBS prior to inoculation onto HEYM slopes (100 µl per slope) without further dilution in order to determine the presence of any M. paratuberculosis cells recovered by IMS. This experiment was repeated four times.
Comparison of the recovery of a fixed number of M. paratuberculosis cells by culturing after centrifugation alone, centrifugation and IMS, and centrifugation and decontamination with 0.75% HPC. In previous M. paratuberculosis milk surveys (18, 19) the workers centrifuged and decontaminated the milk samples with 0.75% HPC before preparations were cultured on HEYM slopes. A study was carried out to compare the numbers of M. paratuberculosis cells recovered by culturing after centrifugation and IMS and by culturing after centrifugation and HPC decontamination from different volumes of milk (1, 5, 10, and 50 ml) inoculated with approximately 106 CFU of M. paratuberculosis/ml. Culturing after centrifugation alone was included as a control. Control milk samples were centrifuged at 2,500 × g for 15 min, and each pellet was resuspended in 1 ml of sterile water. IMS milk samples were centrifuged and resuspended in 1 ml of PBS prior to IMS as described above. IMB were resuspended after IMS in 1 ml of sterile water. For decontamination, milk samples were centrifuged, resuspended in 5 ml of 0.75% HPC, and incubated at room temperature for 4 h with occasional shaking. HPC-treated samples were then centrifuged again, and each pellet was resuspended in 1 ml of sterile water. All of the samples were then diluted as necessary and inoculated onto HEYM slopes (100 µl per slope). The slopes were incubated for up to 12 weeks, and colony counts were obtained.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Confirmation of attachment of M. paratuberculosis to coated IMB. Fluorescent microscopy revealed that M. paratuberculosis cells attached to the IMB coated with purified rabbit anti-M. paratuberculosis IgG. It was evident that large clumps, not just single cells, were bound to some IMB, and often more than one cell or clump of cells were attached to the same IMB or group of beads (Fig. 2).
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Specificity of purified rabbit anti-M. paratuberculosis polyclonal IgG. The polyclonal IgG raised against M. paratuberculosis B4 produced strong agglutination reactions with all M. paratuberculosis strains available for testing in our laboratory (a total of 10 strains were tested, including 2 type strains and 8 field strains that originated from laboratories in the United States, Denmark, Northern Ireland, and Scotland). Moderate cross-reactions of the polyclonal IgG with three other Mycobacterium spp. and weak cross-reactions with bacterial isolates from raw milk were observed (Table 1). Table 1 also shows that a 1:1,000 dilution of the polyclonal IgG in PBS still reacted strongly with M. paratuberculosis NCTC 8578, whereas the levels of the cross-reactions with the other Mycobacterium spp. and the milk isolates diminished as the IgG was diluted.
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Determination of optimum immunocapture time.
Immunocapture
times of 15, 30, and 60 min (with gentle agitation) after addition of
10 µl of IMB were investigated. Similar trends were observed for the
two M. paratuberculosis strains tested (NCTC 8578 and
B2). Figure 3 shows how the number of
M. paratuberculosis cells recovered by IMS was affected
by immunocapture time and suspending medium. Overall, the numbers of
M. paratuberculosis cells recovered by IMS from milk
and milk/PBS samples were not significantly different, but the number
of cells recovered from PBS alone was significantly less for both
strains (P < 0.001). The percentage of recovery of
M. paratuberculosis from each of the suspending media,
which was calculated by determining the number of cells attached to the
IMB, was surprisingly low. The highest percentage of recovery (37.1%)
was obtained by incubating inoculated milk for 60 min with IMB, and the
lowest percentage of recovery (
0.2%) was obtained with inoculated
PBS. The optimum immunocapture times for M. paratuberculosis cells varied with the suspending medium, as
follows: whole milk, 30 to 60 min; milk-PBS, 30 min; and PBS, 15 min
(Fig. 3). Subsequently, when the numbers of M. paratuberculosis cells which did not bind to the IMB were determined for a range of milk samples containing 102 to
106 CFU/ml, we found that the IMB had a maximum binding
capacity of between 104 and 105 CFU (Fig.
4). Consequently, significant proportions
of the inoculated M. paratuberculosis population were
effectively lost when milk samples containing >104 CFU
were subjected to IMS. This explains why just 37% of M. paratuberculosis cells were recovered by IMS from milk initially
inoculated with 106 CFU/ml.
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Effect of centrifugation prior to IMS. M. paratuberculosis cells were present in all three milk fractions after centrifugation at 2,500 × g for 15 min. Overall, 13.0, 17.6, and 69.4% of the M. paratuberculosis cells present in a 10-ml milk sample segregated into the cream, whey, and pellet fractions, respectively, after centrifugation at 2,500 × g for 15 min. As the majority of the M. paratuberculosis cells were located in the pellet (P < 0.05), centrifugation was subsequently used to concentrate low numbers of M. paratuberculosis in larger volumes of milk prior to IMS. The numbers of M. paratuberculosis cells recovered by IMS after centrifugation of 5-, 10-, and 50-ml samples of milk inoculated with 106 CFU of M. paratuberculosis did not differ significantly (P > 0.05) (Fig. 5).
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Detection limit of the IMS method. M. paratuberculosis was consistently isolated by the optimized IMS procedure from milk inoculated with 10 CFU/ml when milk samples inoculated with different concentrations of M. paratuberculosis (107 to 10 CFU/ml) were tested on four separate occasions. When centrifugation was used to concentrate the M. paratuberculosis cells in larger volumes of inoculated milk prior to IMS, the limit of detection by the culture method increased to 10 CFU per original volume (5, 10, or 50 ml) of milk tested.
Comparison of methods for the recovery of M. paratuberculosis from milk. Similar numbers of M. paratuberculosis cells were recovered from milk samples by culturing after centrifugation alone and after centrifugation and HPC decontamination irrespective of the initial milk volume (Fig. 5). In contrast, significantly lower numbers of M. paratuberculosis cells were recovered by culturing after centrifugation and IMS (P < 0.001), although similar numbers of cells were recovered by this method from different volumes of milk. The latter finding is explained by the limited binding capacity of the IMB.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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In this paper we describe successful development and optimization of a novel IMS method for isolation of M. paratuberculosis from milk. It was clear from previous IMS studies (3-5, 16, 17, 22) that IMS was not intended for quantification purposes since it was generally used with preenriched samples. Our novel IMS method for M. paratuberculosis isolation should aid in detection, not quantification, of this organism in milk when it is used in conjunction with a suitable end point detection method. The IMS method consistently detected M. paratuberculosis in milk samples inoculated with 10 CFU/ml when it was used in association with culturing on HEYM slopes. This level of detection was possible in the absence of selective preenrichment, which is commonly performed prior to IMS of other food pathogens (4, 5, 22), and therefore indicates that the method is sensitive. The optimum immunocapture time after addition of IMB varied depending on the nature of the medium in which the M. paratuberculosis cells were suspended. The longest immunocapture time (60 min) was that required for whole milk, and the shortest immunocapture time (15 min) was that required for PBS. Our experiments showed that when 10-ml volumes of inoculated milk were centrifuged, the majority (69.4%) of M. paratuberculosis cells segregated in the pellet. Therefore, in future studies involving this IMS method, we will centrifuge 50-ml volumes of milk, resuspend each pellet in 1 ml of PBS-T prior to IMS, and use an immunocapture time of 30 min in order to maximize the sensitivity of the method.
Research groups reporting new IMS methods generally assess the performance of an IMS method in terms of the percentage of recovery obtained with an inoculated population (5, 22). A similar approach was taken in this study, although we readily acknowledge that interpretation of CFU data for M. paratuberculosis is difficult because of the probability that CFU arise from both single cells and clumps of cells. Counts obtained after IMS are semiquantitative at best (3). Examination of bead-cell complexes after IMS by using fluorescent acid-fast staining clearly illustrated that several cells or clumps can be bound to each IMB or cluster of IMB (Fig. 2). Nevertheless, an indication of the capabilities of the new IMS method was obtained. Initially, the percentages of recovery by IMS from milk, milk/PBS, and PBS samples inoculated with 106 CFU of M. paratuberculosis/ml were calculated by counting the M. paratuberculosis cells attached to the IMB. The values obtained were disappointingly low compared with the values given in previously reported IMS studies performed with other food pathogens (5, 22). However, an alternative approach for determining the percentages of recovery of cells by IMS is to enumerate the cells which do not bind to the beads but are lost with the milk after the magnetic separation step. Milk samples inoculated with a range of M. paratuberculosis concentrations (106 to 102 CFU/ml) were examined by taking this alternative approach. The results indicated that 10 µl of IMB (approximately 106 beads) had a maximum binding capacity of 104 to 105 CFU. This meant that when 102 to 104 CFU of M. paratuberculosis was present in a 1-ml milk sample, the percentage of recovery was close to 100% (Fig. 4), whereas when >104 CFU was present in a 1-ml milk sample, a maximum of only 104 CFU could be recovered. Additional evidence that the maximum binding capacity is limited was provided by the finding that the concentrations of M. paratuberculosis recovered after centrifugation and IMS from various volumes of milk that were initially inoculated with 106 to 107 CFU of M. paratuberculosis were consistently around 104 CFU/ml, approximately 100 times lower than the concentrations obtained by culturing after centrifugation and HPC decontamination (Fig. 4). During this study, some batch variation in the binding capacity of the IMB was observed. For example, data in Fig. 3 indicate that the binding capacity approached 106 CFU, whereas data in Fig. 5, which were obtained with a different batch of Dynabeads, indicate that the maximum level of recovery was just over 104 CFU of M. paratuberculosis. The limited binding capacity of the coated IMB is of no real consequence since an accurate determination of the number of M. paratuberculosis cells present in a milk sample is not possible after IMS; in any case, high numbers of M. paratuberculosis would never be encountered in naturally infected milk. The novel IMS method for M. paratuberculosis used in conjunction with culturing gives an indication of the presence or absence of viable M. paratuberculosis cells.
We used polyclonal antibodies raised against radiation-killed M. paratuberculosis to coat magnetic beads in this study. Polyclonal antibodies are directed against a number of surface antigens rather than against a single surface antigen, which avoids the problem of the high level of specificity which can sometimes occur with monoclonal antibodies. It also increases the likelihood of isolating the desired organism. Unfortunately, since some of the surface antigens may not be unique to M. paratuberculosis, there is a possibility of nonspecific cross-reactions with the polyclonal IgG. Slide agglutination confirmed that there were some cross-reactions between the polyclonal IgG and other mycobacteria and milk bacteria (Table 1). We used undiluted polyclonal IgG to coat the sheep anti-rabbit IgG-coated Dynabeads and were generally able to isolate M. paratuberculosis from milk containing 10 CFU/ml initially, so even though the IMS method was not completely specific, it was very sensitive. We found that cross-reactions of the polyclonal IgG with the milk isolates, in particular, were eliminated by diluting the IgG (Table 1). Therefore, it may be possible to improve the specificity of the IMS method by coating magnetic beads with a dilution of the polyclonal IgG (1:100 or 1:1,000). However, using a lower concentration of polyclonal IgG to coat magnetic beads may reduce the sensitivity of the IMS method, and this possibility should be investigated. It may be possible to circumvent this shortcoming in terms of specificity by using IMS in conjunction with BACTEC radiometric medium, to which PANTA antibiotic supplement could be added to combat the growth of contaminants, rather than HEYM. Alternatively, instead of culturing to confirm the presence of M. paratuberculosis, IMS could be used in conjunction with IS900 PCR, which is specific for this organism.
IMS is a relatively simple procedure to perform, although it is a little laborious. However, there is a potential risk that IMB and, therefore, M. paratuberculosis cells may be lost during the washing steps if care is not taken when the supernatant is removed by aspiration between washes. Milk is notorious as a suspending medium which can create problems for IMS applications due to its high fat content (3). Particular care is needed when the supernatant is removed after the first 10 min of magnetic separation. At this stage the IMB tend to slip down the side of the tube as the supernatant is being removed by aspiration rather than being tightly captured on the wall of the tube. However, with each subsequent washing step as the IMB are cleaned and milk components trapped among the IMB are removed, the beads tend to become more tightly captured on the wall of the tube, and there is less likelihood that they will be accidentally discarded.
In summary, we developed and evaluated an IMS procedure for isolating M. paratuberculosis from milk samples. This IMS procedure takes less than 1 h, compared to at least 5 h for HPC decontamination prior to culturing, and was found to consistently result in isolation of M. paratuberculosis cells from milk containing 10 CFU/ml. Centrifugation of larger volumes of milk and resuspension in 1 ml of PBS-T prior to IMS considerably improve the sensitivity of the method. The potential value of this novel IMS method is not for quantification of M. paratuberculosis; rather, it can be used for rapid detection of this organism in milk when it is combined with end point detection methods, such as IS900 PCR or an ELISA (3). In future work we will concentrate on evaluating the use of this novel IMS method in conjunction with IS900 PCR as a rapid technique for screening milk and feces samples for the presence of M. paratuberculosis.
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ACKNOWLEDGMENTS |
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This work was supported by funds from the Ministry of Agriculture, Fisheries and Food, United Kingdom.
We thank Bill Graham for assistance during irradiation of the M. paratuberculosis antigen and Colin Bell, who carried out the ELISA work.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Food Science (Food Microbiology), The Queen's University of Belfast, Newforge Lane, Belfast BT9 5PX, United Kingdom. Phone: 44 1232 255299. Fax: 44 1232 668376. E-mail: I.Grant{at}qub.ac.uk.
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Abstract
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Materials & Methods
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Discussion
References
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Applied and Environmental Microbiology, September 1998, p. 3153-3158, Vol. 64, No. 9
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