Bacterial etiologic agents causing neonatal sepsis and associated risk factors in Gondar, Northwest Ethiopia

A prospective cross-sectional study was conducted among all admitted neonates for sepsis at the University of Gondar Hospital from September/2015 to May/2016. Diagnosis of neonatal sepsis remains challenging in this hospital, and mainly depends on clinical decision.

Neonates with clinical sign and symptoms of sepsis at the time of admission or who develop sepsis during their stay in hospital were included in this study.

Neonates with sepsis, who started antibiotic therapy, were excluded from the study.

Presence of bacterial infection was dependent variable, whereas independent variable were age, sex, occupation, weight at birth, gestational week, mode of delivery, maternal health condition (fever, urinary tract infection), bottle feeding, Apgar score at 5 min, and skin or local infection.

Bacteremia means the presence of bacteria in the blood stream, which may or may not be caused by infectious agents. Septicemia, on the other hand, it is serious disease characterized by systemic signs, and the presence of bacteria and their toxins in the blood stream.

After getting written consent from guardian two bottle of blood samples (1 ml for each bottle) from two different sites of peripheral vein were collected aseptically (disinfecting with 70% alcohol and 2% tincture of iodine) by experienced nurses prior to any antibiotic use. The collected blood sample was inoculated directly into Trypton soya broth blood culture medium bottles (Oxoid LTD) and sent to the medical microbiology laboratory for culture and drug susceptibility testing. The blood cultures were incubated aerobically at 37 °C and observed daily for the first 3 days for the presence of visible microbial growth by one of the following: haemolysis, air bubbles (gas production), and coagulation of broth. At the same time, subcultures were made during successive days on enriched and selective media including blood agar plate (Oxoid LTD), chocolate agar plat (incubated at 5% CO₂ atmosphere), MacConkey (Oxoid Ltd. Basingstoke, Hampshire, UK), and manitol salt agar plates and examined for growth after 24–48 h of incubation.

The same protocol was repeated until the 7th day before blood cultures were considered to be free of microorganisms. Isolates obtained were identified by standard microbiological techniques namely, Gram staining, colony characteristics, and biochemical properties including catalase, coagulase (free and bound), growth on manitol salt agar, and hemolytic activity on blood agar plate for Gram positive isolates, and triple sugar iron, motility, indole, citrate utilization, urease, oxidase and H2S production for Gram negative isolates [20]. As described above two aerobic blood culture bottles were used for each patient, and growth in both bottles was considered as positive. Thus, growth of bacteria only from one bottle did not regard as pathogen and considered as contamination.

Antimicrobial susceptibility test was carried out for each identified bacteria based on Clinical and Laboratory Standard Institute guideline by using disc diffusion method on Muller Hinton agar for non-fastidious organisms and Muller Hinton agar with 5% defibrinated sterile sheep blood for fastidious organisms [21].

Three to five pure colony of the test organism was taken by using a sterile wire loop and emulsify in 2 ml of nutrient broth. The bacterial suspensions turbidity was matched and checked with 0.5 McFarland standards. Then a sterile cotton swab was dipped in to the suspension and squeeze free from excess fluid against the side of test tube. The test organisms were uniformly seed on the surface of Muller-Hinton agar for non fastidious group and Muller Hinton agar with 5% defibrinated sterile sheep blood for fastidious group and expose to a concentration gradient of antibiotic diffusing from antibiotic impregnated paper disc into the agar medium and the medium was incubated at 35 °C for 18–24 h [22].

The following antimicrobial disks were used (Oxoid UK), Amoxicillin-clavulanate (AMC:20/10 μg), penicillin (P:10 unit), trimethoprim-sulfamethoxazole (SXT:1.25/23.75 μg), erythromycin (E:15 μg), tetracycline (TE: 30 μg), clindamycin (DA:2 μg), chloramphenicol (CAF:30 μg), ampicillin (AMP:10 μg), gentamicin (CN:10 μg), amikacin (AK:30 μg), ciprofloxacin (CIP: 5 μg), ceftazidime (CAZ: 30 μg),ceftriaxone (CRO:30 μg) and cefoxitin (CXT:30 μg). Grades of susceptibility pattern were interpreted by comparison of the zone of inhibition according to Clinical and Laboratory Standard Institute 2014 guideline [21].

All materials, equipment and procedures were adequately controlled. Pre-analytical, analytical and post-analytical stages of quality assurance that are incorporated in standard operating procedures of the medical microbiology laboratory were strictly followed. The sterility of culture media was ensured by incubating 5% of each batch of the prepared media at 37^oc for 24 h. Performance of all prepared media was also checked by inoculating international standard-strains such as E.coli (ATCC 25922) Gram negative bacteria, S. aureus (ATCC 25923) for Gram positive bacteria and N. gonorrhoeae (ATCC49226) for fastidious bacteria. To standardize the inoculums density of bacterial suspension for the susceptibility test, 0.5 McFarland standards was used [20]. To ensure the accuracy of data, double data entry method was used.

Of the total study participants (n = 251), 149 (59.4%) were male, 184 (73.3%) of the neonates were age ≤ 3 days (early onset) and146 (58.2%) were from urban residence. Of the total neonates 46 (18.3%) had very low birth weight (< 1.5 kg), 92 (36.6%) were preterm (<37 week gestation), 160 (63.7%) were delivered by spontaneous vaginal delivery. It was observed that 55 (21.9%) of the neonates mothers had history of urinary tract infection (UTI) during gestational period (Table 1).

Of the study participants with neonatal septicemia, 117 (46.62%) showed bacterial growth and of these 120 different kinds of bacterial pathogens were identified. Three of blood cultures (2.5%) showed mixed growth (poly microbial), while the 114 (97.5%) showed non duplicate growth. The rest 134 (53.4%) had no bacterial growth. Gram positive bacterial species were commonly isolated 81 (67.5%) than the Gram negative bacterial species 39 (32.5%). The commonly isolated bacteria were S. aureus 49 (40.9%) followed by CoNS 26 (21.7%) and K. pneumoniae 19 (15.8%) (Table 2).

The predominant organisms during the first 3 days of life were Gram positive, accounting for 57 (65.5%) of the 87 (72.5%) isolates. Between 3 and 28 days of life, Gram negative and Gram positive isolates accounted for 9 (27.28%) and 24 (72.72%) of the 33 isolated organisms, respectively. The single predominant Gram positive organism in both age groups was S. aureus 49 (40.83%). Among Gram negatives, K. pneumonia 19 (15.83%) was the predominant causative agent in both age groups (Table 2).

From the total isolates only 11 (9.2%, 95% CI, 4.4–15%) isolates were susceptible to all tested antibiotics. Over all in Gram positive isolates high resistance rate were observed to penicillin 42 (51.8%), ampicillin 30 (37%) and trimethoprim- sulfamethoxazole 34 (42%). On the other hand, Gram positive bacteria showed least resistance rate to clindamycin 7 (8.6%) andciprofloxacin 16 (19.7%). As indicated Table 3, species specific antibiotic resistance rates showed that more than 35% of S. aureus isolates were resistant to penicillin, ampicillin, Trimethoprim- sulfamethoxazole, gentamicin anderythromycin.

Susceptibility pattern in Gram negative isolates indicates that high susceptibility rate seen in amikacin 37 (94.9%), ciprofloxacin, ceftazidamide and gentamicin each 34 (87.2%) and highly resistance seen in ampicillin 33 (84.6%), ceftriaxone 22 (56.4%) and trimethoprim/ sulfamethoxazole 17 (43.58%). Species specific antibiotic resistance in Gram negative has also indicated, E.coli were resistant to ampicillin 8 (66.7%) but relatively no resistance rates were noted to ciprofloxacin and amikacin. K. pneumonia was highly resistance to ampicillin 18 (94.75%), ceftriaxone 15 (78.9%) and trimethoprim/sulfamethoxazole 8 (42.1%). It was highly sensitive to ciprofloxacin and gentamicin 16 (84.2%) each (Table 4).

Among the total isolates, 78 (65%, 95% CI: 56.7–72.5%) were resistance to three or more different class of antibiotics. Among MDR strains, 21 (17.5%) isolate were resistant to three classes of antibiotics, the rest 57 (47.5%) were resistant to greater than three classes of antibiotics. Result of drug resistance patterns compared within species specific showed that, 33 (67.3%) of S. aureus, 8 (66.7%) of E. coli and 16 (84.2%) of K. pnuemonae were MDR isolates. Among the total isolates of S. aureus, 13 (26.5%) of them were found to be MRSA (Table 5).

Risk factors associated with neonatal septicemia were analyzed. Univariate and multivariate analysis showed that very low birth weight with adjusted odds ratio (AOR) 12.37 (95% CI: 4.135–37.04), low birth weight with AOR 2.63 (95% CI: 1.149–6.09),caesarean section mode of delivery with AOR 5.2(95% CI: 2.36–11.37), Apgar score < 7 with AOR 0.438 (95% CI: 0.215–0.892) and preterm gestational week with AOR 8.99 (95% CI: 4.175–19.38) were associated with neonatal septicemia (Table 6).

Multivariate analysis result indicates that gestational week has significant association which means that neonates born in gestation < 37 weeks had almost nine times more likely to develop sepsis compared to those neonates born in gestation ≥37 weeks. Neonates born with very low birth weight < 1.5 kg had 12 times more likely to develop neonatal sepsis as compared to normal birth weight > 2.5 kg. Neonates born with birth weight < 2500 Gram had 3 times more likely to develop sepsis than neonates with normal birth weight. Apgar score < 7 pre five minute had 0.5 times more likely to develop sepsis than neonates with normal Apgar score. Caesarian section mode of delivery had 5 time risk to develop neonatal sepsis than spontaneous vaginal delivery.

A specific characterization MDR bacterium (MRSA, ESBL) has not been done due to lack of well-established methodological techniques. Moreover, molecular based specification for some bacterial groups (CoNS) was not done.