Bacteremia associated with naturally occurring acute coliform mastitis in dairy cows
John R. Wenz, DVM, MS; George M. Barrington, DVM, PhD, DACVIM; Franklyn B. Garry, DVM, MS, DACVIM;
Kevin D. McSweeney, BS; R. Page Dinsmore, DVM, DABVP; Gregory Goodell, DVM;
become the predominant form of mastitis in herds inwhich contagious mastitis has been effectively con-
Objective—To determine the incidence of bacteremia
trolled.1-3 Despite decades of research focused on ACM,
in dairy cows with naturally occurring acute coliform
wholly effective control measures have yet to be estab-
mastitis (ACM) with a wide range of disease severity.
lished, and proper treatment of the disease remains
Design—Cohort study.
controversial. Our understanding of ACM pathophysi-
Animals—144 dairy cows with ACM from 6 herds.
ology is based largely on studies of the experimental
Procedure—Cows were examined at time of identifi-
disease model. These studies typically involved inocu-
cation of ACM (time 0) and classified as having mild,
lation of a healthy mammary gland with coliform
moderate, or severe mastitis on the basis of rectal
organisms (Aerobacter aerogenes, E coli, and Klebsiella
temperature, hydration status, rumen contraction rate,
spp) or with purified endotoxin. Results of these
and attitude. Cows were reexamined at 24 or 48 hours.
experiments suggest coliform bacteria are noninvasive,
Bacteriologic culturing of milk and blood (30 ml), CBC,
and bacteremia (the presence of bacteria in the circu-
and serum biochemical analysis were performed at
lating blood) is not considered a significant sequela to
each time point. Appropriate samples were obtained at
ACM.4-6 Furthermore, disease manifestation has been
a single point from herdmates without mastitis (con-
primarily attributed to the effects of endotoxin.
trols) that were closely matched for lactation number
Consequently, it has been widely held that antibiotic
and days since parturition. Blood culture results werecompared among severity groups and controls by use
therapy is not warranted in cases of ACM. We feel that
of χ2 tests, as was outcome of an ACM episode for
studies of naturally occurring ACM will help resolve
cows grouped by blood bacterial isolates.
discrepancies between knowledge based on the exper-
Results—Bacteria were isolated from 52 blood samples
imental disease model and practitioner experience in
from 46 of 144 (32%) cows with ACM, which was signif-
icantly more than control cows (11/156; 7.1%). Group-1
In 1 study7 of 20 cases of naturally occurring ACM,
isolates (Escherichia coli, Pasteurella multocida,
only Bacillus spp were isolated from a few cases, a find-
Mannheimia haemolytica, Klebsiella pneumoniae,
ing that was attributed to skin contamination. The
Enterobacter agglomerans, and Salmonella enterica
severity of disease was not clearly defined, only one 5-
serotype Typhimurium) were identified in 20 of 144 (14%)
ml blood sample was evaluated, and controls were not
cows with ACM and 0 of 156 control cows. Group-1 iso-
included in the study. In our previous work,8 the exis-
lates were identified in 4.3, 9.1, and 42% of cows classi-
tence of bacteremia associated with naturally occurring
fied as having mild, moderate, and severe ACM, respec-tively. Escherichia coli and K pneumoniae milk and blood
ACM was established, in which bacteremia associated
isolates obtained from the same cow were of the same
with E coli was identified in 32% (11/34) of cows with
genotype. Bacillus spp were identified in 21 of 144 (15%)
severe protracted coliform mastitis. That study, howev-
cows with ACM, which was significantly more than con-
er, lacked controls and was limited to a select popula-
trol cows (3/156; 1.9%). Thirty-five percent of cows with
tion of cows with severe protracted disease.
a group-1 isolate died during the mastitis episode.
Furthermore, it has been suggested that bacteremia
Conclusions and Clinical Relevance—Results sug-
observed in these cows may have been the result of pro-
gest that bacteremia develops in a substantial pro-
tracted disease rather than specific to the ACM
portion of cows with ACM. Classification of severity
episode.6 Recently, we have reported important patho-
of disease is important for establishment of effective
physiologic differences among cows with ACM grouped
treatment protocols; parenteral antimicrobial treat-
ment may be indicated in cows with ACM. (J Am Vet
The purposes of the study reported here were to
determine the incidence of bacteremia in dairy cows
Acute coliform mastitis (ACM), typified by with naturally occurring ACM and a wide range of dis- Escherichia coli intramammary infection, has
ease severity, determine whether the affected mamma-ry gland was the source of bacteremia, and identify fac-
From the Department of Clinical Sciences, College of Veterinary
tors that may be useful in predicting the occurrence of
Medicine, Colorado State University, Ft. Collins, CO 80523. Dr.
Barrington’s present address is Washington State University,Department of Veterinary Clinical Sciences, College of Veterinary
Materials and Methods
Supported by the Colorado Agricultural Experiment Station,
Herds—Cows at 6 dairies surrounding Fort Collins,
Pharmacia Animal Health, and The American Association of
Colo, that developed clinical mastitis between July 1997 and
January 1999 were eligible for inclusion in the study. During
The authors thank Jane Carmen for technical assistance.
the study, there were approximately 4,000 Holstein cows in
lactation at the 6 dairies. Cows were fed a total mixed ration
agar plates. Plates were incubated at 37 C in an atmosphere
(TMR) in groups based on production level and were milked
containing 10% CO2 and examined after 24 and 48 hours.
in a parlor 3 times daily. All cows were housed in drylot pens
Bacterial colonies were identified in accordance with
or freestalls. Mean somatic cell count of bulk tank milk was
National Mastitis Council guidelines.10 Coliform intramam-
< 300,000 cells/ml throughout the study period for all dairies.
mary infection was diagnosed if samples contained ≥ 10
All cows were vaccinated with a bacterin containing the J-5
colony-forming units (cfu) of at least 1 coliform organ-
strain of E colia at the start of the nonlactating period and 4
ism/ml. Plates with ≥ 3 organisms were considered contami-
weeks before and within 2 weeks after parturition. Heifers
nated. Bacterial numbers obtained following culture were
received the J-5 bacterin 2 weeks before and within 2 weeks
reported as < 10,000, 10,000 to 100,000, and > 100,000
after parturition. All dairies practiced effective contagious
mastitis control programs and participated in a program for
Blood was collected from the jugular vein of cows with
monthly bacterial culture of bulk tank milk samples.
ACM at time 0 and 24 hours later or at time 0 and 48 hourslater and submitted for bacterial culture. Blood from control
Inclusion criteria and data collection—Farm personnel
cows was collected at a single time point. Hair was shaved,
identified cows as possibly having coliform mastitis if 1 or
using a disposable razor, and the skin was disinfected with at
more of the following signs were present: reduced milk pro-
least 3 alternating applications of povidone iodine scrub and
duction, abnormal milk, and 1 or more abnormal mammary
70% ethanol at a site over the jugular vein. Thirty milliliters
quarters. Initial examination and sample collection (time 0)
of blood was aseptically drawn from the vein into a 35-ml
was performed by 1 of the authors (JRW, KM), usually with-
syringe through an 18-ga needle. Fifteen milliliters of blood
in an hour after notification from the farm. Cows identified
was injected aseptically through a new 18-ga needle into each
with mastitis during the evening or night milking were exam-
of two 50-ml blood culture vials of brain-heart infusion broth
ined the following morning. Farm personnel treated cows
containing 0.6% sodium polyanetholsulfonate.b Samples were
according to established farm protocols after initial examina-
aerated through a filtered needle and incubated at 37 C in an
tion and sample collection by study personnel. Treatment
atmosphere containing 10% CO2. Samples were subcultured
was not controlled in order to maximize producer participa-
onto blood agar on days 0, 1, and 7 and incubated at 37 C in
tion in the study and determine the incidence of bacteremia
an atmosphere containing 10% CO2. Plates were examined for
associated with ACM given current varied farm treatment
growth and recorded at 24 and 48 hours. Escherichia coli, K
protocols. Treatment among farms was consistent in the use
pneumoniae, Pasteurella multocida, Mannheimia haemolytica,
of anti-inflammatory drugs (flunixin meglumine, phenlybu-
tazone), 7.2% sodium chloride solution (administered IV),
Typhimurium isolates were considered to be important path-
and electrolyte solutions (administered PO). Antimicrobial
ogenic bacteria and were classified as group-1 isolates.
therapy varied among and within farms and included com-
Environmental streptococci, coagulase-negative staphylococ-
mercially available antibiotic preparations (intramammary),
ci, and Acinetobacter spp were considered to be coincidental
gentamicin (intramammary), dexamethasone (intramamma-
findings and classified as group-2 isolates. Bacillus spp were
ry), ceftiofur (IV and IM), and oxytetracycline (IV).
Secretions were removed from affected mammary glands 3times a day at the time of milking and an additional 2 times
Coliform isolate genotyping—Genotyping of E coli and
a day during treatments. Cows for which bacterial culture of
K pneumoniae was performed on isolates obtained from milk
a milk sample yielded E coli or Klebsiella spp were included
and blood of the same cow as described previously.11
in the study. Healthy herdmates, closely matched to infected
Enterogenic repetitive intergenic consensus sequence
cows by lactation number and days since parturition, were
primers were used to perform polymerase chain reaction (PCR) on the genomic DNA of E coli and K pneumoniae iso-
Cows were evaluated at the time of initial examination
lates. The presence and size (base pairs) of PCR products
(time 0) and again 24 hours later or at time 0 and again 48
were compared between milk and blood coliform isolates
hours later. Control cows were examined at 1 of the time
points. Age, lactation number, days since parturition, rectaltemperature, heart rate, respiratory rate, and rumen contrac-
Hematologic testing—Blood samples were collected
tion rate were recorded. Hydration status was estimated on
from the tail vein at time 0 and 24 hours later or time 0 and 48
the basis of degree of enophthalmos and scored as 0 (none),
hours later. Testing of blood from control cows was not per-
1 (mild enophthalmos), 2 (moderate enophthalmos), or 3
formed, because laboratory reference ranges were already
(severe enophthalmos). Attitude was classified on the basis
established. Samples anticoagulated with EDTA were used for
of signs of depression as none, mild, or severe.
CBC and determination of plasma protein and fibrinogen con-centrations. Samples collected in plain tubes without anticoag-
Severity classification—Cows with ACM were classi-
ulant were used to harvest serum, and serum glucose, creati-
fied as having mild, moderate, or severe disease on the basis
nine, total protein, albumin, globulin, total bilirubin, phos-
of rectal temperature, hydration status, rumen contraction
phorus, calcium, magnesium, sodium, potassium, chloride,
rate, and attitude at time 0 (Appendix).
and bicarbonate concentrations; aspartate transaminase, γ-glu-tamyltransferase, sorbitol dehydrogenase, and creatine kinase
Bacteriologic culture—Secretions from affected mam-
activities; and anion gap were determined. Hematologic values
mary glands were collected at time 0 and 24 hours later or
were compared between cows with a group-1 bacteremia and
time 0 and 48 hours later and submitted for bacterial culture.
those in which blood culture results were negative or a
A composite sample of milk from all quarters of control cows
non–group-1 bacteremia within each severity group.
was collected at a single time point. Teat ends were disinfect-ed with 70% ethanol prior to sample collection, and samples
Outcome—Survival and retention in the herd following
were collected in sterile vials. Samples were stored on ice for
the episode of mastitis were assessed to determine outcome.
transport to the laboratory and processed the day of collec-
Cows that died during the episode of mastitis were classified
tion, except that those submitted to the laboratory after 5:00
as nonsurvivors; all others were considered survivors. Cows
PM were frozen at –4 C and processed the following day.
leaving the herd as a direct result of mastitis (ie, because of
Samples were mixed gently by inverting the tube, and 100 µl
mastitis or low production) within 30 days after the episode
of each sample was plated on blood agar and MacConkey
of mastitis were classified as culled. Cows still present in the
herd 30 days after the episode of mastitis were classified as
single blood sample from 8 cows and in combination
with Bacillus spp in 4 cows with ACM. Bacillus spp
Data analyses—Continuous variables (days since partu-
alone were identified in a single blood sample of 14 cows
rition, age, lactation, and results of clinicopathologic tests)
with ACM. Bacteria were isolated from 30, 8, and 14
were tested for normality by use of the Kolmogorov D statis-
blood samples of cows with ACM taken at 0, 24, and 48
tic. Normally distributed continuous variables were com-
hours, respectively. Bacteria were isolated from the
pared among groups (mild, moderate, or severe disease) by
blood of cows with ACM at both 0 and 24 hours from 3
use of ANOVA. Continuous variables that were not normally
cows and at both 0 and 48 hours from 3 cows. Group-1
distributed were compared among groups by use of
isolates were identified at time 0 in 11 cows, at 24 hours
Wilcoxon rank sum or Kruskal-Wallis tests. Categorical vari-
in 3 cows, at 48 hours in 4 cows, at 0 and 24 hours in 1
ables (milk bacterial count, proportion of bacteremic cows)
cow, and at 0 and 48 hours in 1 cow. Cows were classi-
were compared among groups by use of χ2 tests, except thatFisher exact tests were used when the expected count in
fied as bacteremic if bacteria were isolated from at least
> 25% of the categories was < 5. Influence of farm on blood
1 blood sample at any time point. Group-1 bacteremia
culture results and outcome data was evaluated by use of a
was identified in a significantly (P < 0.001) greater per-
maximum-likelihood ANOVA procedure.c Statistical calcula-
centage of cows with ACM (14%; 20/144), compared
tions were performed by use of commercially available soft-
with control cows (0%; 0/156). Fifteen percent (21/144)
ware.c Relative risk was calculated as an odds ratio; the odds
of cows with ACM had a Bacillus spp bacteremia, which
ratio was not considered significantly different from 1 if its
was significantly (P < 0.001) more than control cows
95% confidence interval included 1. For all other tests, val-
(1.9%; 3/156). The percentage of cows with group-2 iso-
ues of P < 0.05 were considered significant.
lates was not significantly (P = 0.2) different betweencows with ACM and controls.
Samples were collected from 178 cows with sus-
When evaluated on the basis of severity of ACM, a
pected ACM. Cows were excluded if samples yielded
significantly greater percentage of cows in the severe
no growth on 0-hour milk culture (n = 13), a noncol-
group had a group-1 bacteremia (42%), compared with
iform organism was isolated (n = 15), or the 0-hour
moderate (9.1%) and mild (4.3%) groups (Table 1). In
milk sample was contaminated (n = 2). Four cows were
contrast, significant differences were not detected in
excluded because data necessary for severity classifica-
the percentage of cows with group-2 or Bacillus spp
isolates among severity groups. The odds of a group-1bacteremia in cows in the severe group were 15 (95%
Bacteriologic testing—Coliform organisms were confidence interval [CI], 4.1 to 61.9) and 7.2 (95% CI,
isolated from the time-0 milk culture of 144 cows that
2.1 to 25.2) times greater than in cows in the mild and
were subsequently enrolled in the study. Organisms
included E coli (n = 122), K pneumoniae (n = 19), and
Group-1 bacteremia was identified in a significant-
3 cases in which both E coli and K pneumoniae were
ly greater percentage of cows with > 100,000 cfu/ml in
milk from the infected gland at time 0 (23%; 15/64)
Bacteria were isolated from 52 blood samples in 46
than in cows with < 100,000 cfu/ml (5.3%; 4/76).
of 144 (32%) cows with ACM, which was significantly
Significant differences in cfu/ml bacteria in milk from
(P < 0.001) more than those isolated from 11 of 156
the infected gland were not detected in cows with
(7.1%) control cows. Group-1 isolates (E coli, K pneu-
group-2 or Bacillus spp isolates alone. moniae, Pasteurella multocida, Mannheimia haemolytica,E agglomerans, and Salmonella Typhimurium), group-2
Coliform isolate genotyping—Genotyping was
isolates (environmental streptococci, coagulase nega-
performed on coliform organisms of the same genus
tive staphylococci, and Acinetobacter spp), and Bacillus
isolated from the milk and blood of the same cow.
spp isolates were evaluated independently. Group-1
Escherichia coli was isolated from the milk and blood of
isolates alone were identified in a single blood sample
10 cows, and K pneumoniae was isolated from the milk
from 14 cows, in combination with a group-2 isolate in
and blood of 1 cow. The DNA fingerprint of E coli milk
2 cows, and in combination with Bacillus spp in 4 cows
and blood isolates, obtained from the same cow, had
with ACM. Group-2 isolates alone were identified in a
the same banding pattern, indicating they were the
Table 1—Number and percentage of positive blood culture results by bacterial isolate from cows withacute coliform mastitis classified by severity of disease and control cows
Group-1 Group-2 Bacillus isolates isolates isolates Severity (n)
Values within a column with different superscripts are significantly (P Ͻ 0.05) different. Blood bacterial isolates were eval-
uated independently; therefore, cows with more than 1 isolate type were counted more than once.
Group-1 isolates = Escherichia coli, Pasteurella multocida, Mannheimia hemolytica, Klebsiella pneumoniae, Enterobacter
agglomerans, Salmonella Typhimurium. Group-2 isolates = Environmental streptococci, coagulase-negative staphylococci,and Acinetobacter spp.
Table 2—Survival and retention rates in a group of 144 cows with acute coliform mastitis
Negative Group-1 Group-2 Bacillus culture result isolates isolates No. % No. % No. % No. %
*Values were significantly (P Ͻ 0.001) different. Cows were grouped according to results of bacteriologic culture of blood.
Comparisons were only made between groups of isolates and cows with negative culture results; comparisons were notmade between bacteremic groups.
Died = No. of cows that died during the mastitic episode. Retained = No. of cows still present in the herd 30 days after the
mastitic episode. Culled = No. of cows removed from the herd as a direct result of mastitis.
same genotype. The K pneumoniae milk and blood iso-
tured (Table 1). Antimicrobial use was variable among
lates from the same cow were also of the same genotype.
and within farms and may have had an impact onresults of this study. Therefore, the proportion of bac-
Differentiation of group-1 bacteremic cows and
teremic cows may be higher in cases of ACM that are
cows with negative blood culture results or non–group-1 bacteremia—Signalment and hematologic
Intermittent bacteremia is commonly the result of
data were compared between cows with group-1 bac-
bacterial infiltration of the blood through the lymphatics
teremia and those with negative blood culture results or
from a site of localized infection.12 It has been suggested
non–group-1 bacteremia within each severity group.
that the E coli bacteremia observed by Cebra et al8 may
Significant differences were not detected in mean number
have been nonspecific and attributable to prolonged
of days since parturition, age, and lactation number of
severe disease. Indeed, E coli isolated from the blood
cows with group-1 bacteremia versus those without by
samples in that study could have come from the large
severity group.9 Complete hematologic data were available
pool in the gastrointestinal tract. However, antibiotic sen-
for 141 cows. Median values of CBC and serum biochem-
sitivity patterns of E coli isolated from milk and blood of
ical analysis by severity group have been reported. 9 There
the same cow were similar, which suggests a common
were no significant differences in hematologic values of
source. Furthermore, in the present study, genotyping by
cows with group-1 bacteremia versus those without by
use of PCR indicated that E coli and Klebsiella spp isolat-
severity group. Significant and clinically important differ-
ed from blood were the same as those isolated from the
ences did exist in the severity classification of cows with
mammary gland of the same cow, indicating the infected
group-1 bacteremia versus those without (Appendix).
mammary gland was the likely source of bacteremia.
Sixty-five percent (13/20) of cows with group-1 bac-
Resident macrophages in the liver and spleen are
teremia were classified as severe, compared with only 15%
primarily responsible for bacterial clearance of the
(18/122) of those without group-1 bacteremia.
blood; however, bacterial opsonization and subsequent
Outcome—Outcome was evaluated based on sur-
phagocytosis by circulating leukocytes play a role as
vival through the mastitic episode and retention on
well.13 Leukopenia, specifically neutropenia, has been
farm for 30 days following the episode (Table 2). No
well documented in cows with ACM. Furthermore,
significant differences in the percentage of cows that
results from our previous work revealed that cows with
died or were culled were observed between cows with
more severe systemic disease signs have more pro-
a group-2 isolate or Bacillus spp isolate versus cows
found neutropenia,9 which may increase the probabili-
with negative blood culture results. A significantly (P <
ty of obtaining positive blood culture results in cows
0.001) greater percentage (35%) of cows with a group-
with more severe ACM. Indeed, cohort studies of
1 isolate died, compared with cows with negative
immunocompromised humans have demonstrated a
blood culture results or a non-group 1 isolate (0%).
positive relationship between neutropenia and bac-
Significant differences in culling were not observed
teremia attributable to gram-negative bacilli such as E
among cows grouped by blood culture results.
coli and Klebsiella spp.14 However, although it wasreported that a significant difference was not detected
Discussion
in median neutrophil count in cows with moderate
Results of this study indicated bacteremia develops
versus severe systemic disease signs,9 results of the pre-
in a substantial proportion of cows with naturally
sent study indicated there were significantly more pos-
occurring ACM. Furthermore, bacteremia caused by
itive blood culture results obtained from cows with
group-1 pathogens (E coli, P multocida, M haemolytica,
severe ACM (48%), compared with cows with moder-
K pneumoniae, E agglomerans, and Salmonella
ate ACM (23%). Furthermore, despite the profound
Typhimurium) develops in a significant proportion of
neutropenia observed in cows with moderate ACM,
cows with ACM and is associated with severity of sys-
compared with those with mild ACM,9 there was no
temic disease signs. Our results also revealed that a sig-
difference in positive blood culture results between the
nificantly greater percentage of cows in the mild and
2 groups (Table 1). The same was true when only
moderate groups had group-1 bacteremia, compared
group-1 blood isolates were considered. Our results
with controls from which no group-1 isolates were cul-
suggest that a factor other than neutropenia may be
involved in the pathophysiology of bacteremia associ-
severity groups, all cows with Bacillus spp bacteremia
survived, and there was no difference in cull rate, com-
Many factors may have been responsible for failure
pared to cows with negative blood culture results.
to identify bacteremia associated with ACM in previous
Group-2 isolates (ie, environmental streptococci,
studies.5-7 Most used experimental disease models in
coagulase-negative staphylococci, and Acinetobacter
which the mammary glands of healthy cows were
spp) were considered inconsequential, as there was no
inoculated with a specified uniform number of col-
difference between controls and cows with ACM.
iform bacteria. Disease manifestation is thought to be
Furthermore, there was no difference in outcome
the result of interaction of host, pathogen, and envi-
between cows with a group-2 isolate alone and those
ronmental factors. Epidemiologic studies4,15,16 of ACM
with negative blood culture results. Group-2 isolates
have indicated that E coli is an accidental pathogen
may have been contaminants or present in the blood of
with no specific virulence factors involved in establish-
ing infection of the mammary gland. Furthermore,
Blood cultures were performed at 2 time points to
despite the consistency of inoculum size and control of
increase the chance of identifying cows with bac-
environmental factors afforded by the experimental
teremia. The second time point was 24 hours after ini-
model, pathophysiologic response varies widely among
tial examination (time 0) at the start of the study; how-
individual cows.16 Taken together, these results suggest
ever, it was later changed to 48 hours. The 48-hour
cow factors (ie, immune status, presence of concurrent
time point allowed for better evaluation of changes in
disease, teat-end condition) may be most important in
hematologic data; furthermore, results of our previous
determining the pathogenesis of ACM. Therefore, con-
study identified bacteremia in cows that were ill for a
siderable differences in disease manifestation may exist
median of 48 hours.8 Interestingly, 65% (13/20) of
in the experimental disease of healthy cows that
cows with group-1 positive blood culture results were
arguably have intact host defenses versus naturally
identified at time 0, and 35% (7/20) were in the mild
occurring disease in cows that are likely to have com-
or moderate group. This is further evidence that the
observed bacteremia was not merely the result of
Recently we reported that severity classification
based on systemic disease signs effectively distin-
The design of this study did not allow for discrim-
guished significant pathophysiologic differences
ination of the cause-and-effect relationship between
among cows with ACM.9 Previous studies that failed to
severity of disease and bacteremia. However, evaluation
identify bacteremia did not evaluate or clearly define
of the data collected suggests that bacteremia caused by
severity of ACM cases. Results of the present study
group-1 pathogens had a negative impact on cows with
indicated that group-1 bacteremia develops in a signif-
ACM. Death during the mastitis episode only occurred
icantly smaller proportion of cows with mild and mod-
in cows with group-1 bacteremia. Six of 7 cows that
erate disease signs, compared to cows with severe dis-
died were in the severe group, suggesting severity of an
ease signs (Table 1). Consequently, a predominance of
ACM episode is an important factor. Severe disease
more mildly affected cows combined with a small sam-
alone, however, does not appear to determine survival.
ple size may have resulted in failure to identify bac-
Seven of 13 severely affected cows with group-1 bac-
teremia survived, compared with 18 of 18 severely
Culture technique may account for failure to iden-
affected cows without group-1 bacteremia. Together,
tify bacteremia associated with ACM. Previous studies
these data suggest group-1 bacteremia was an added
typically performed blood culture on 5 ml of blood col-
insult to severe disease that resulted in a poorer out-
lected at a single time point. Often < 10 bacteria are
come. Severe disease, however, is not a prerequisite for
present per milliliter of blood in intermittently bac-
development of group-1 bacteremia, as 35% of group-1
teremic human patients.17 The chances of obtaining a
bacteremic cows were in the mild and moderate groups.
positive culture are directly related to the volume of
However, of cows with mild and moderate disease
blood collected.18 Increasing the blood volume collect-
severity, only 1 of 7 (a cow in the moderate group) with
ed from 2 ml to 20 ml resulted in an increase in posi-
tive cultures from 30% to 50% in human patients,18-20
The culling rate of surviving cows was the same in
whereas volumes > 30 ml did not result in a significant
cows with ACM regardless of blood culture results
increase in positive yield.20 When sequential blood cul-
(Table 2). Likewise, of the cows with severe disease
tures were performed in humans that did not have
that survived, there was no difference in culling
endocarditis, 80% were positive on first culture, 90%
between cows with group-1 bacteremia (57%; 4/7) and
after second culture, and 99% after third culture.18 In
those without (61%; 11/18). Therefore, it appears that
the present study, 30-ml blood samples were collected
group-1 bacteremia has a negative impact on survival
at 2 time points in an attempt to optimize identifica-
but not culling during the first 30 days following a
Bacillus spp have been isolated from blood in pre-
Pasteurella multocida or Mannheimia haemolytica
vious studies but were presumed to be skin contami-
was isolated from the blood of 7 cows, E agglomerans
nants.6-8 Inclusion of controls in the present study indi-
from 1 cow, and Salmonella Typhimurium from 1 cow
cates Bacillus spp bacteremia is 8 times more likely in
with ACM. These bacteria were not, however, isolated
cows with ACM, compared with controls. The signifi-
on milk culture of the same cow. These findings sug-
cance and source of Bacillus spp bacteremia in cows
gest some cases of bacteremia associated with coliform
with ACM is unclear. The incidence was similar among
mastitis may be the result of bacterial translocation
from other organ systems. Cows with Pasteurella or
acute coliform mastitis in Holstein cattle. J Vet Intern Med 1996;
Mannheimia spp bacteremia had more severe disease
signs, and their prognosis was grave. These bacteria are
9. Wenz JR, Barrington GM, Garry FB, et al. Use of systemic
disease signs to assess severity in dairy cows with acute coliform
normal flora of the upper portion of the respiratory tract
mastitis. J Am Vet Med Assoc 2001;218:567–572.
of cattle and are involved in the bovine respiratory dis-
10. National Mastitis Council. Laboratory handbook on bovine
ease complex. Studies in sheep and in vitro studies of
mastitis. Madison, Wis: National Mastitis Council Inc, 1999;31–39.
bovine pulmonary endothelial monolayers indicate that
11. Lipman LJA, de Nijs A, Lam TJGM, et al. Identification of
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blood of 5 of 9 cows with naturally occurring ACM. 23
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antimicrobial therapy may be indicated in such casesof ACM. Appendix Scheme based on systemic disease signs for classifying sever-
aJ-5 Bacterin, Pharmacia and Upjohn Animal Health, Kalamazoo,
ity of acute coliform mastitis in dairy cows*
bBBL, Becton Dickinson Co, Cockeysville, Md. Variable Criteria
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*Cows with total score of 0 to 2 were classified as having mild disease,
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cows with total score of 3 to 5 were classified as having moderate disease,
and cows with total score of 6 to 9 were classified as having severe disease.
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From: Cocaine and Methamphetamine Addiction: Treatment, Recovery, and Relapse Prevention. By A.M. Washton & J.E. Zweben. Norton Professional Books, 2009. Copyrighted. Chapter 3 Stimulant Drugs and Sex Many stimulant users report that their use of cocaine or methamphetamine is strongly associated with sex. Male users in particular report that stimulant drugs increase their libi