AIM: To determine serum IL-1beta, IL-6, IL-8, and TNF-alpha levels in neonatal sepsis at the time of diagnosis and after therapy, and to show the meaningful on the follow up. METHODS: This prospective study was performed on newborns who were hospitalized for neonatal sepsis and who were classified as culture-proven sepsis (n=12), as culture-negative sepsis (n=21), and as healthy newborns (n=17). RESULTS: At the time of diagnosis, serum IL-1beta, IL-6, IL-8, and TNF-alpha levels of culture-proven sepsis were significantly higher than those of the control groups (P<.05). At the time of diagnosis, IL-1beta, IL-6, IL-8, and TNF-alpha levels of culture-proven sepsis and culture-negative sepsis were significantly higher than levels at the seventh day after antibiotic treatment. CONCLUSION: Serum IL-1beta, IL-6, IL-8, and TNF-alpha are mediators of inflammation and can be used at the diagnosis and at the evaluation of the therapeutic efficiency in neonatal sepsis.
AIM: To determine serum IL-1beta, IL-6, IL-8, and TNF-alpha levels in neonatal sepsis at the time of diagnosis and after therapy, and to show the meaningful on the follow up. METHODS: This prospective study was performed on newborns who were hospitalized for neonatal sepsis and who were classified as culture-proven sepsis (n=12), as culture-negative sepsis (n=21), and as healthy newborns (n=17). RESULTS: At the time of diagnosis, serum IL-1beta, IL-6, IL-8, and TNF-alpha levels of culture-proven sepsis were significantly higher than those of the control groups (P<.05). At the time of diagnosis, IL-1beta, IL-6, IL-8, and TNF-alpha levels of culture-proven sepsis and culture-negative sepsis were significantly higher than levels at the seventh day after antibiotic treatment. CONCLUSION: Serum IL-1beta, IL-6, IL-8, and TNF-alpha are mediators of inflammation and can be used at the diagnosis and at the evaluation of the therapeutic efficiency in neonatal sepsis.
Bacterial
infection in newborns, especially preterm, may rapidly evolve into generalized
sepsis. This condition has a gradual and subtle onset, with nonspecific symptoms
that may severely compromise the infant’s clinical state if untreated and lead
to life-threatening consequences. Neonatal sepsis has a fairly low incidence at
birth (1–10/1000 live births) but may affect up to 16% of infants in the
neonatal intensive care unit (NICU) with birth weight of 501–1500 gm. The mortality rate is very high: 15–50% of affected infants [1].Clinical
manifestations are nonspecific and laboratory parameters such as white blood
cell (WBC) count or C-reactive protein (CRP) are of limited value in identifying
infected newborns. As a consequence, appropriate diagnosis and therapy could be
delayed, worsening the prognosis of the patient [2-6].In
studies elsewhere [4,7,8], the WBC count showed a low detection sensitivity in
neonatal infection. Even the combination of total neutrophil count, immature-to-total
neutrophil ratio (I/T), and platelet count failed to reach an appropriate sensitivity
and specifity in this pathology. C-reactive protein has been thoroughly studied
as a diagnostic tool in neonatal sepsis and also as an indicator of response to
therapy [9, 10].The underdeveloped immune system
predisposes preterm newborns to infection, which is a major cause of neonatal
morbidity and mortality. Sepsis and endotoxin activate monocytes, macrophages,
lymphocytes, fibroblasts, and endothelial cells that produce and secrete IL-1, TNF-,
-interferon, IL-6, IL-8, and other proinflammatory cytokines. IL-6,
stimulated by TNF-, IL-1, and endotoxin of viral and bacterial infections,
acts as a T-cell activation indicator, induces antibody secretion by human
B-cells, causes differentiation of cytotoxic T-cells, and also has the ability
to inhibit TNF- production. Moreover, IL-6 is the major stimulant in hepatic
protein synthesis, that is, CRP and fibrinogen during acute phase responses.
Previous studies have shown that determinations of IL-6 in neonatal blood are of
diagnostic value in sepsis. Elevated serum IL-1, IL-6, IL-8, and TNF- levels have been
found in both the neonatal and adult sepsis. Several studies have evaluated the
role of cytokine determinations as early diagnostic markers in neonatal sepsis
[11-17].The
aim of this study is to determine serum IL-1, IL-6, IL-8, and TNF- levels in
neonatal sepsis at the time of diagnosis and after therapy and to show the
meaningful on the follow up.
2. MATERIAL AND METHODS
This prospective study was performed on newborns who were hospitalized for neonatal
sepsis at NICU. Inclusion criteria were positive clinical signs of sepsis
and/or history of factors associated with increased risk for infection and
parental informed consent. Exclusion criteria were congenital malformations,
congenital infections associated with the TORCH complex, and refusal of
parental consent. Clinical signs of sepsis were defined as the presence of three
or more of the following categories of clinical signs: apnea, tachypnea
(60/min), nasalflaring, retraction, cyanosis, respiratory distress-bradycardia
(100/min), tachycardia (180/min), hypotonia, seizures-poor skin colour,
capillary refilling time longer than two seconds, irritability, and lethargy. Historical
factors associated with increased risk for infection included premature rupture
of the membranes (in term infants 18 hours), maternal fever during labour, intraamniotic
infection, and chorioamnionitis.
Two or more abnormal values of the sepsis screen (as white blood cell count
4000 or 10.000 mm3, immature-to-total neutrophil ratio
higher than 0.2 and CRP positivity) were considered as supportive for diagnosis
of infection [18]. Newborns were classified as culture-proven sepsis (positive
blood culture), as culture-negative sepsis (negative blood culture, but
clinical signs of sepsis with positive sepsis screen and/or a history of risk
factors, and antibiotic treatment longer than 7 days), and as control groups (healthy,
noninfectious newborns). Blood samples were obtained at time of diagnosis and seventh day after
antibiotic treatment, their serum extracted and IL-1, IL-6, IL-8, and TNF- were determined.Blood
analysis was done in Firat Medical Center Immunology Laboratory (Elazig, Turkey). The local
ethics commission approved the study.CRP was determined by the Behring
Nephelometer 100 Analyzer BN II (NY, USA). Detection limit was 3 mg/L and a
serum value of 8 mg/L was defined as
abnormally elevated. The serum samples
of the study and control groups were studied by ELISA for IL-1, IL-6, IL-8,
and TNF- levels with human cytokine kits (Biosource, Calif, USA). Detection
limit for serum IL-1 level was 1 pg/mL, measure range was 0–250 pg/mL. Detection limit for serum IL-6 level was 2 pg/mL,
measure range was 0–500 pg/mL. Detection limit for serum IL-8 level was 5 pg/mL,
measure range was 0–1000 pg/mL. Detection limit for serum TNF- level was 1.7 pg/mL, measure range was 0–1000 pg/mL The collected blood samples were
centrifuged at 2500 g for 10 minutes at C. The serum
layer was separated and frozen at C for
cytokine analysis, which was performed in less than 2 weeks. Freezing/thawing
cycles were avoided.Statistical
analyses were performed using the SPSS 11.0 programs for Windowns XP. The
results were done as mean standard deviation. Kruskal Wallis and post hoc test
Scheffe procedures
were used; the difference in three groups and was considered
to be significant. Wilcoxon test was used for the interpretation of the
difference between at time of diagnosis and after therapy.
3. RESULTS
In
total, 50 newborns were included in the study: 12 culture-proven sepsis, 21
culture-negative sepsis, and 17 control. Table 1 shows the characteristics of
the study group.
Table 1
Characteristics of the study groups.
Character
Culture-proven sepsis (n=12)
Culture-negative sepsis (n=21)
Controls (n=17)
Gender M/F
8/4
9/13
8/9
Weight(g)
2033±938
2111±975
2294±761
Gestational age (weeks)
34.2±4.0
34.0±3.3
35.3±2.6
At
time of diagnosis, serum IL-1, IL-6, IL-8, and TNF- levels of culture-proven
sepsis were significantly higher than those of the control groups ();
but only serum IL-8 levels of culture-proven sepsis was significantly higher
than culture-negative sepsis ().At
time of diagnosis, serum IL-1, IL-6, IL-8, and TNF- levels of culture-proven
sepsis and culture-negative sepsis were significantly higher than levels at
seventh day after antibiotic treatment ().Serum
IL-1, IL-6, IL-8, and TNF- levels were showed in Table 2.
Table 2
Serum IL-1, IL-6, IL-8, and TNF- levels of the study groups.
Serum cytokine levels
Culture-proven sepsisa (n=12)
Culture-negative sepsisb (n=21)
Controlsc (n=17)
*P value <.05
IL-1β (pg/mL)
At time of diagnosis1
41.20±13.57
33.30±8.62
10.35±2.65
a-c, b-c
7th day2
10.87±4.49
9.47±3.53
IL-6 (pg/mL)
At time of diagnosis1
193.95±74.11
155.42±70.06
8.19±5.84
a-c, b-c
7th day2
9.45±6.96
8.99±6.08
IL-8 (pg/mL)
At time of diagnosis1
481.33±186.58
376.85±96.61
55.51±26.54
a-b, a-c, b-c
7th day2
89.41±57.69
53.57±34.84
TNF-α (pg/mL)
At time of diagnosis1
21.00±9.43
17.64±6.70
4.55±1.52
a-c, b-c
7th day2
5.23±1.74
4.92±1.68
**P value
P<.05
1-2
1-2
—
—
* Kruskal Wallis test.
** Wilcoxon test.
4. DISCUSSION
Bacterial
infection continues to be the major cause of morbidity and mortality in the
newborn. Because the prognosis for sepsis largely depends on early identification
and treatment, these newborns are subjected to extensive diagnostic evaluation
and empirical systemic antibiotic treatment, pending laboratory results. The definitive
diagnosis of sepsis is made by a positive blood culture, which requires a
minimum of 48–72 hours, yields a positive result in only 30–70% of cases, and
may not always be available in peripheral health centers. Several studies have
examined the laboratory findings associated with sepsis [19-21]. There is,
however, a lack of consensus on the essential tests that would identify
newborns with acute infection. Fowlie et al. [22] conducted a systematic review
to determine the value of diagnostic tests for bacterial infection in early
life (from birth to 90 days old) and reported that the accuracy of tests varies
enormously and the tests are of limited value in the diagnosis of infection.Hematological
parameters have been evaluated in previous studies. Da Silva et al. [23] found
significant heterogeneity across these studies. The possible sources of
heterogeneity were population, age, whether the subjects were at term or
preterm, methodological quality, different leukocyte indices, different cutoff
values, and interpretation of test results by different laboratory observers.In
the past few decades, it has been observed that several mediators of
inflammation tend to become elevated during sepsis. The concentrations of some
proinflammatory cytokines, especially TNF-, IL-6, and IL-8, in systemic circulation
were reported to increase in severe infections and septic shock [24]. Martin et
al. [17] showed that serum IL-6, IL-8, and TNF- levels were all higher in
septic than in nonseptic newborns.The study of IL-1 and TNF-, cytokines that
are synthesized at the beginning of the inflammatory cascade has rendered
differing results. In our study, the serum TNF- and IL-1 levels were significantly
increased in newborns with sepsis. Results of different published studies
relation to these cytokines are contradictory. Concerning IL-1 results,
similar to ours, they
have been reported by some researchers while not by others [25-28]. Publishing
data regarding TNF- is also divergent. Some studies found the diagnostic
utility of this cytokine [25, 26] while others demonstrated similar or even
lower levels in infected newborns compared to healthy newborns [29, 30]. Discrepancies
in results among different studies could be explained by the variations in
laboratory methods in performing the analysis, the time of the sample
collection, or the control population selected [28].Interleukin-6
has been reported as an early indicator of neonatal sepsis because of its rapid
increase after endotoxin challenge. IL-6 is secreted by monocytes and
macrophages in response to bacteremia [31]. Previous studies have shown IL-6 to
be a useful marker of early infection in the newborn [31-34]. Kantar et al. [31]
showed that septic preterm newborns had significantly elevated IL-6 levels at
the onset of sepsis as compared to the recovery period and the controls. In our
study, it was observed that IL-6 levels of newborn with culture-proven sepsis
and culture-negative sepsis were significantly higher than controls ().Interleukin-8
is a cytokine that has a role in the release, activation, and chemotaxis of
neutrophils. Serum IL-8 level has been reported to increase in neonatal sepsis
and have a sensitivity of about 80–90% and a specifity of about 76–100% [35, 36].
In this study, it was detected that IL-8 levels of newborns with culture-proven
sepsis were significantly higher than culture-negative sepsis and controls (). Kocabas et al. [37] and Martin et al. [17] found that IL-8 were
higher in septic than in nonseptic newborns.Another
characteristic of the markers that are used in the diagnosis of neonatal sepsis
is that it gives information about the prognosis of the disease and helps in
coming to a decision as to whether to stop or continue antibiotic treatment. In
this study, it is found that IL-1, IL-6, IL-8, and TNF- levels were
statistically decreased in newborns after seven-day therapy than in newborns at
the time of diagnosis (). Similar results have been obtained
in many studies [37-39].
5. CONCLUSION
Serum levels of IL-1, IL-6, IL-8, and TNF-
are mediators of inflammation and can be used at the diagnosis and at the
evaluation of the therapeutic efficiency in neonatal sepsis.
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