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2. BanLec-eGFP Chimera as a Tool for Evaluation of Lectin Binding to High-Mannose Glycans on Microorganisms

Author

Zorana Lopandić, Luka Dragačević, Dragan Popović, Uros Andjelković, Rajna Minić, and Marija Gavrović-Jankulović

Subjects
banana lectin, eGFP, fluorescence, viral glycoproteins, influenza vaccine, florescence-linked lectin sorbent assay, Microbiology, QR1-502
Abstract

Fluorescently labeled lectins are useful tools for in vivo and in vitro studies of the structure and function of tissues and various pathogens such as viruses, bacteria, and fungi. For the evaluation of high-mannose glycans present on various glycoproteins, a three-dimensional (3D) model of the chimera was designed from the crystal structures of recombinant banana lectin (BanLec, Protein Data Bank entry (PDB): 5EXG) and an enhanced green fluorescent protein (eGFP, PDB 4EUL) by applying molecular modeling and molecular mechanics and expressed in Escherichia coli. BanLec-eGFP, produced as a soluble cytosolic protein of about 42 kDa, revealed β-sheets (41%) as the predominant secondary structures, with the emission peak maximum detected at 509 nm (excitation wavelength 488 nm). More than 65% of the primary structure was confirmed by mass spectrometry. Competitive BanLec-eGFP binding to high mannose glycans of the influenza vaccine (Vaxigrip®) was shown in a fluorescence-linked lectin sorbent assay (FLLSA) with monosaccharides (mannose and glucose) and wild type BanLec and H84T BanLec mutant. BanLec-eGFP exhibited binding to mannose residues on different strains of Salmonella in flow cytometry, with especially pronounced binding to a Salmonella Typhi clinical isolate. BanLec-eGFP can be a useful tool for screening high-mannose glycosylation sites on different microorganisms.

Published
2021
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3. Profiling of microorganism-binding serum antibody specificities in professional athletes.

Author

Rajna Minić, Zlatko Papić, Brižita Đorđević, Danica Michaličkova, Vesna Ilić, Geir Mathiesen, Irena Živković, Visnja Pantic, and Ljiljana Dimitrijević

Subjects
Medicine, Science
Abstract

The goal of this work was to elucidate similarities between microorganisms from the perspective of the humoral immune system reactivity in professional athletes. The reactivity of serum IgG of 14 young, individuals was analyzed to 23 selected microorganisms as antigens by use of the in house ELISA. Serum IgM and IgA reactivity was also analyzed and a control group of sex and age matched individuals was used for comparison. The obtained absorbance levels were used as a string of values to correlate the reactivity to different microorganisms. IgM was found to be the most cross reactive antibody class, Pearson's r = 0.7-0.92, for very distant bacterial species such as Lactobacillus and E. coli.High correlation in IgG levels was found for Gammaproteobacteria and LPS (from E. coli) (r = 0.77 for LPS vs. P. aeruginosa to r = 0.98 for LPS vs. E.coli), whereas this correlation was lower in the control group (r = 0.49 for LPS vs. P. aeruginosa to r = 0.66 for LPS vs. E.coli). The correlation was also analyzed between total IgG and IgG subclasses specific for the same microorganism, and IgG2 was identified as the main subclass recognising different microorganisms, as well as recognising LPS. Upon correlation of IgG with IgA for the same microorganism absence of or negative correlation was found between bacteria-specific IgA and IgG in case of Lactobacillus and Staphylococcusgeni, whereas correlation was absent or positive for Candida albicans, Enterococcusfaecalis,Streptococcus species tested in professional athletes. Opposite results were obtained for the control group. Outlined here is a simple experimental procedure and data analysis which yields functional significance and which can be used for determining the similarities between microorganisms from the aspect of the humoral immune system, for determining the main IgG subclass involved in an immune response as well as for the analysis of different target populations.

Published
2018
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4. Impact of Tree Pollen Distribution on Allergic Diseases in Serbia: Evidence of Implementation of Allergen Immunotherapy to Betula verrucosa

Author

Rajna Minić, Mirjana Josipović, Vesna Tomić Spirić, Marija Gavrović-Jankulović, Aleksandra Perić Popadić, Ivana Prokopijević, Ana Ljubičić, Danijela Stamenković, and Lidija Burazer

Subjects
aerobiology, betula verrucosa, pollination, allergic disorders, allergen immunotherapy, Medicine (General), R5-920
Abstract

Background and objectives: The relationship between air pollen quantity and the sensitization of allergic patients is crucial for both the diagnosis and treatment of allergic diseases. Weather conditions influence the distribution of allergenic pollen and increases in pollen concentration may negatively affect the health of allergic patients. The aim of this study was to analyze the implementation of allergen immunotherapy with regard to air pollen concentration. Material and Methods: Here we examined the relationship between Betula air pollen concentration and the usage of Betula verrucosa allergen immunotherapy in Serbia. Examination covered the period from 2015 to 2018. Measurement of airborne pollen concentration was performed with Lanzoni volumetric pollen traps. The evidence of the usage of sublingual allergen immunotherapy (SLIT) was gathered from patients with documented sensitization to specific pollen. Results: During this period tree pollens were represented with 58% ± 21% of all measured air pollen species, while Betula pollen represented 15% ± 8% of all tree pollens. Betula pollination peaked in April. Allergen immunotherapy to Betula verrucosa in Serbia is entirely conducted as sublingual immunotherapy and represents 47.1% ± 1.4% of issued tree pollen SLIT. The use of pollen SLIT increased by 68% from 2015 to 2018, with an even greater increase in usage recorded for Betula SLIT—80%. Conclusions: This analysis shows a clear causative relationship between pollination and the type/prevalence of applied allergen immunotherapy. Information about the flowering seasons of allergenic plants is very important for people who suffer from allergy, for clinical allergologists, as well as for governing authorities. The presented data is of practical importance to the proper timing of immunotherapy initiation and of importance for urban landscaping. The obtained data can be the starting point for the instatement of a thorough epidemiological study and the inclusion of Serbia on the pollen map of Europe.

Published
2020
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6. Comparison of Enzyme-Linked Lectin Sorbent Assay and Flow Cytometry for Profling Microbial Glycans

Author

Luka Dragačević, Zorana Lopandić, Marija Gavrović-Jankulović, Irena Živković, Veljko Blagojević, Natalija Polović, and Rajna Minić

Subjects
0303 health sciences, Glycosylation, Plant lectins, 030302 biochemistry & molecular biology, Microorganisms, Reproducibility of Results, Musa, Bioengineering, General Medicine, Flow Cytometry, Applied Microbiology and Biotechnology, Biochemistry, Salmonella Lactobacillus, 03 medical and health sciences, Polysaccharides, Lectins, Yeasts, Plant Lectins, Molecular Biology, 030304 developmental biology, Biotechnology
Abstract

The surface of microorganisms is covered with carbohydrates, which makes them unique, self-sustaining glycan probes. Lectins are able to bind to these probes, and this interaction can be exploited for selecting microorganisms or novel lectins. To examine lectin-microorganism interactions, we have previously developed an enzyme-linked lectin sorbent assay (ELLSA) with whole bacterial cells. To further test the validity of this methodology, here we compare it with flow cytometry. For this purpose, we used biotinylated recombinantly produced lectin from Musa acuminata (BanLec), this lectin’s recombinantly produced chimera with green fluorescent protein (BanLec-eGFP) and a lectin from Ricinus communis (RCA120), both biotinylated and FITC labeled. Parallel testing showed equivalent results for the two methods, in terms of the presence or absence of binding, with signal intensity yielding high Pearson correlation coefficient of 0.8 for BanLec and 0.95 for RCA120. The ELLSA method demonstrated multiple advantages, such as reliability and convenience for high-throughput analysis; it also required less lectin and yielded more consistent results. As such, ELLSA proved to be a useful tool for profiling microbial glycan structures or testing novel lectins. Supplementary material: [https://cherry.chem.bg.ac.rs/handle/123456789/4888]

Published
2022

7. Selectivity of polyclonal repertoire of anti-microbial IgA and its subclasses in saliva and serum in humans

Author

Slavomir Nikodijević, Veljko Blagojević, Ivana Ćuruvija, Dejana Kosanović, Tamara Djukić, Brižita Djordjević, Vesna Ilić, and Rajna Minić

Subjects
Immunology, Immunoglobulins, Enzyme-Linked Immunosorbent Assay, General Medicine, Immunoglobulin A, salivary IgA, Immunoglobulin A, Secretory, Escherichia coli, serum IgA, Humans, Saliva, microorganisms, IgA, IgA subclasses
Abstract

Increased interest in microbiota calls for the thorough analysis of antibody reactivity to different microorganisms. As salivary IgA represents the first line of defence against microorganisms contacting mucosal surfaces, we explored the binding and specificity of salivary IgA by testing the binding of purified, FITC-labelled salivary IgA to different microorganisms in flow cytometry and conclude that this kind of analysis enables the differentiation of species/strains with high IgA binding capacity, which should be corroborated on a larger sample size. Further we compare, with in-house ELISA, the binding of polyclonal salivary IgA with the binding of polyclonal serum IgA from the same individuals to whole microbial cells and to purified microbial components. High correlations were obtained in total salivary IgA binding to Lactobacillus rhamnosus and Escherichia coli, very distant bacterial species, as well as to isolated bacterial components (r = .70–.97). The binding of total salivary IgA resembled the binding of both salivary IgA1 and IgA2, with IgA2 predominating. For serum polyclonal IgA repertoire, substantially higher specificity was obtained. Serum IgA binding to E. coli correlated best with serum IgA binding to lipopolysaccharide (r = .86), and serum IgA against L. rhamnosus correlated best with the anti-peptidoglycan IgA levels (r = .88). We have also detected that total serum IgA response is governed by either IgA1 or IgA2 response, depending on the nature of the antigen/s. We conclude that steady state salivary IgA repertoire, unlike serum IgA repertoire, consists of polyreactive antibodies with innate specificity, questioning its capacity to select resident microbiota.

Published
2022

9. MTT based L-aminoacid oxidase activity test for determination of antivenom potency against Vipera ammodytes envenomation

Author

Jelena Vakic, Vitomir Ćupić, Vladimir Milovanovic, Saša Ivanović, Rajna Minić, Sunčica Borozan, Irena Zivkovic, and Andrijana Nešić

Subjects
0106 biological sciences, MTT, Antivenom, venom, Hemorrhage, Venom, Viper Venoms, Toxicology, 01 natural sciences, complex mixtures, Vipera ammodytes venom, 03 medical and health sciences, Microtiter plate, Viperidae, Animals, Potency, MTT assay, Envenomation, 0303 health sciences, Oxidase test, Vipera ammodytes, biology, Potency test, Antivenins, Chemistry, 010604 marine biology & hydrobiology, 030302 biochemistry & molecular biology, biology.organism_classification, Biochemistry, L-Amino acid Oxidase monomer, Oxidoreductases
Abstract

The MTT assay is routinely used to detect the activity of living cells. While working with Vipera ammodytes venom we detected the reduction of MTT without the presence of cells, in a concentration-dependent manner. By combining non-reducing PAGE, L-amino acid oxidase (LAAO) assays, and standard MTT assays, we established and confirmed that venom MTT reduction is catalyzed by only one enzyme, the LAAO. Even though it was previously known that the dimeric and tetrameric forms of LAAO are active, we conclude that the enzyme is also active in the monomeric form. Our results have led to the definition of a new MTT assay in a microtiter plate for in vitro testing of svLAAO activity i.e. from the venom of the V. ammodytes snake. Potentially, this method can be used for testing hemorrhagic venoms of other snakes as well as the LAAO neutralization capability of appropriate antivenoms.

Published
2021

10. The effect of influenza vaccine immunization on natural antibodies

Author

Ljiljana Dimitrijević, Vladimir Petrušić, Lina Muhandes, Irena Živković, and Rajna Minić

Subjects
0301 basic medicine, Pharmacology, Influenza vaccine, Pharmaceutical Science, Biology, biochemical phenomena, metabolism, and nutrition, immunization, immune homeostasis, RS1-441, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Immune system, Pharmacy and materia medica, natural antibodies, Immunization, Vaccination status, Antigen specific, Immunology, biology.protein, Acquired immune response, bacteria, Immune homeostasis, Antibody, 030215 immunology
Abstract

Natural, polyreactive, low-affinity antibodies are known to play an important role not only in the immediate defense against pathogens, but also in shaping the acquired immune response. On the other hand, antigen specific, high-affinity antibodies can affect the balance of natural antibodies and lead to autoimmune diseases. In this study, we have analyzed the changes that occur in the IgM and IgG pool of natural antibodies after immunization with split or whole virion influenza vaccine. For this purpose, "in-house" developed ELISAs were used. The subjects were divided, according to the vaccination status, into those who had been immunized with the influenza vaccine in previous years and those who had been immunized for the first time. The analysis indicated that the pool of natural antibodies was not impaired by the immunization, evidenced by the lack of changes in any of the groups, and that certain fluctuations were induced in order to maintain the homeostasis of the immune system.

Published
2021

11. Optimization, Validation and Standardization of ELISA

Author

Rajna Minić and Irena Zivkovic

Subjects
0301 basic medicine, 03 medical and health sciences, 030104 developmental biology, Standardization, Computer science, 010401 analytical chemistry, InformationSystems_INFORMATIONSTORAGEANDRETRIEVAL, 01 natural sciences, GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries), 0104 chemical sciences, Reliability engineering
Abstract

The enzyme-linked immunosorbent assay (ELISA) is a commonly used analytical immunochemistry assay based on the specific bond between the antigen and the antibody. The application of this test has significantly changed the practice of medical laboratories in which it is used for detection and quantification of molecules such as hormones, peptides, antibodies, and proteins. Various technical variants of this test can detect antigen (native or foreign) or antibody, determine the intensity of the immune response whether pathological or not; the type of induced immune response as well as the innate immunity potential; and much more. These capabilities, as well as the high sensitivity and robustness of the test and a small price, make it possible to quickly and reliably diagnose diseases in most laboratories. Besides, ELISA is a test that is also used in veterinary medicine, toxicology, allergology, food industry, etc. Despite the fact that it has existed for almost 50 years, different ELISA tests with different technical solutions are still being developed, which improves and expands the application of the this exceptional test. The aim of this chapter is to empower the rider to optimize, standardize and validate an enzyme linked immunosorbent assay.

Published
2020

12. Contributors

Author

Abdullah, Mohd Ibrahim, Abou-Kheir, Wassim, Agrawal, Ojaskumar D., Ahmad, Aryati, Aleksandra, Arsic, Alghamdi, Badrah, Algindan, Yasmin, Almikhlafi, Mohannad A., Alp, Esma Keleş, Alstadhaug, Karl Bjørnar, AlZaim, Ibrahim, Amani, Reza, Ariyanfar, Shadi, Aschner, Michael, Ashraf, Ghulam Md, Bajaj, Komal K., Bakkar, Nour-Mounira Z., Barone, Michele, Bhatti, Gurjit Kaur, Bhatti, Jasvinder Singh, Bitarafan, Sama, Bjerring, Emilie L., Bloomfield, Frank, Buckett, Lauren, Buoite Stella, Alex, Cabañas, Ericka, Cadet, Patrick, Carollo, James J., Castles, Zoe, Chacón, Marina, Chamaa, Farah, Chaudhary, Sameer, Chaudhary, Sapana, Clarke, Evan G., Contreras, Irazú, Cormack, Barbara, Costa, Edbhergue Ventura Lola, Cruz, George B., Cuervo-Zanatta, Daniel, Dangat, Kamini, Darwish, Batoul, De Leo, Sabrina, Dearborn-Tomazos, Jennifer L., Dhandapani, Manju, Dhandapani, Sivashanmugam, Doehner, Wolfram, El Idrissi, Abdeslem, El-Mallah, Carla, El-Yazbi, Ahmed F., Emenike, Bright U., Esposito, Dario, Estrada, José A., Farahbakhsh, Payam, Feldman, Eva L., Gaikwad, Anil B., Gaio, Marina, Gigliotti, Federica, Gordon, Shaileigh, Graneri, Liam, Gulati, Sheffali, Harirchian, Mohammad Hossein, Heath, Rory J., Heffernan, Aaron, Hernandez-Acosta, Julieta, Heyn, Patricia C., Ibeh, Stanley, Iqbal, Asma, Jahromi, Soodeh Razeghi, Jauert, Nadja, Jiang, Leanne, Joseph, Jewel N., Joshi, Sadhana, Julian, Thomas Henry, Kalayeh, Hamed Mirzaei Ghazi, Kale, Mayur B., Kanozia, Rubal, Khattab, Rabie, Kim, Bhumsoo, Klevebro, Susanna, Kloster, Alix H., Kobeissy, Firas, Kraeuter, Ann-Katrin, Kulkarni, Yogesh A., Lam, Virginie, Li, Shuai Cheng, Li, Yinhu, Liampas, Andreas, Longhitano, Calogero, López-Granero, Caridad, Mamo, John C.L., Manganotti, Paolo, Manorenj, Sandhya, Marde, Vaibhav S., Marinelli, Sara, Markowitz, Morri E., Mastrangelo, Mario, Mehrabani, Sanaz, Mekawy, Narmin, Mishra, Jayapriya, Mohamadinarab, Maryam, Morales, Mónica, Navik, Umashanker, Neigh, Gretchen N., Neuwirth, Lorenz S., Ngo, Shyuan T., Nogueira, Romildo de Albuquerque, Norouzy, Abdolreza, Oda, Adriana Leico, Olesen, Margrethe A., Oza, Manisha J., Patel, Vinood B., Perez-Cruz, Claudia, Pessoa, Daniella Tavares, Prasanan, Jayashri, Preedy, Victor R., Quintanilla, Rodrigo A., Rafiee, Pegah, Rajendram, Rajkumar, Rajna, Minic, Rawat, Sakshi, Reddy, P. Hemachandra, Rumora, Amy E., Salvioni, Cristina C.S., Sánchez-Santed, Fernando, Sánchez-Valle, Vicente, Sarnyai, Zoltan, Savelieff, Masha G., Sehrawat, Abhishek, Shaik, Reshma Sultana, Sharma, Eva, Silva, Jeine Emanuele Santos da, Simone, Isabella Laura, Simonsen, Axel Meyer, Soltani, Danesh, Sondhi, Vishal, Steyn, Frederik J., Tagawa, Alex, Tai, Mei-Ling Sharon, Takechi, Ryusuke, Taksande, Brijesh G., Terhune, Elizabeth, Togha, Mansoureh, Tzoulis, Charalampos, Umare, Mohit D., Umekar, Milind J., Upaganlawar, Aman B., Vasquez, Michelle A., Wankhede, Nitu L., White, Hayden, Wilson, Mitchell, Wood, Thomas R., Yamagata, Kazuo, Yi, You Gyoung, Zhu, Wei, Zis, Panagiotis, and Zorica, Stevic

Published
2023
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13. Immunogenic Properties of Lactobacillus plantarum Producing Surface-Displayed Mycobacterium tuberculosis Antigens

Author

Vincent G. H. Eijsink, Lise Øverland, Geir Mathiesen, Harald Carlsen, Charlotte R. Kleiveland, Rannei Tjåland, Rajna Minić, Katarzyna Kuczkowska, Tor Lea, and Lars F. Moen

Subjects
0301 basic medicine, Tuberculosis, 030106 microbiology, Applied Microbiology and Biotechnology, Microbiology, immunology, Mycobacterium tuberculosis, 03 medical and health sciences, Mice, Immune system, Antigen, medicine, Animals, Tuberculosis Vaccines, Immunity, Mucosal, LAB, Antigens, Bacterial, Ecology, biology, biology.organism_classification, medicine.disease, Immunoglobulin A, lactic acid bacteria, Mice, Inbred C57BL, mucosal vaccine, 030104 developmental biology, tuberculosis, Female, bacteriology, Tuberculosis vaccines, BCG vaccine, Bacteria, Lactobacillus plantarum, Food Science, Biotechnology
Abstract

Tuberculosis (TB) remains among the most deadly diseases in the world. The only available vaccine against tuberculosis is the bacille Calmette-Guérin (BCG) vaccine, which does not ensure full protection in adults. There is a global urgency for the development of an effective vaccine for preventing disease transmission, and it requires novel approaches. We are exploring the use of lactic acid bacteria (LAB) as a vector for antigen delivery to mucosal sites. Here, we demonstrate the successful expression and surface display of a Mycobacterium tuberculosis fusion antigen (comprising Ag85B and ESAT-6, referred to as AgE6) on Lactobacillus plantarum . The AgE6 fusion antigen was targeted to the bacterial surface using two different anchors, a lipoprotein anchor directing the protein to the cell membrane and a covalent cell wall anchor. AgE6-producing L. plantarum strains using each of the two anchors induced antigen-specific proliferative responses in lymphocytes purified from TB-positive donors. Similarly, both strains induced immune responses in mice after nasal or oral immunization. The impact of the anchoring strategies was reflected in dissimilarities in the immune responses generated by the two L. plantarum strains in vivo . The present study comprises an initial step toward the development of L. plantarum as a vector for M. tuberculosis antigen delivery. IMPORTANCE This work presents the development of Lactobacillus plantarum as a candidate mucosal vaccine against tuberculosis. Tuberculosis remains one of the top infectious diseases worldwide, and the only available vaccine, bacille Calmette-Guérin (BCG), fails to protect adults and adolescents. Direct antigen delivery to mucosal sites is a promising strategy in tuberculosis vaccine development, and lactic acid bacteria potentially provide easy, safe, and low-cost delivery vehicles for mucosal immunization. We have engineered L. plantarum strains to produce a Mycobacterium tuberculosis fusion antigen and to anchor this antigen to the bacterial cell wall or to the cell membrane. The recombinant strains elicited proliferative antigen-specific T-cell responses in white blood cells from tuberculosis-positive humans and induced specific immune responses after nasal and oral administrations in mice.

Published
2016

14. Intestinal carriage of vancomycin‐resistant Enterococcus spp. among high‐risk patients in university hospitals in Serbia: first surveillance report

Author

Ana Janjusevic, Ljiljana Markovic Denic, Rajna Minic, Anita Grgurevic, and Ivana Cirkovic

Subjects
VRE carriage, MLVA sreening, Antibiotic susceptibility, Serbia, Therapeutics. Pharmacology, RM1-950, Infectious and parasitic diseases, RC109-216, Microbiology, QR1-502
Abstract

Abstract Background The screening for intestinal carriage of vancomycin-resistant Enterococcus spp. (VRE) among high risk patients in the Balkan region and molecular epidemiology of VRE is insufficiently investigated, yet it could be of key importance in infection control. The aim of this study was to provide baseline data on VRE intestinal carriage among high-risk patients in Serbian university hospitals, to determine the phenotypic/genotypic profiles of the isolated VRE, to obtain knowledge of local resistance patterns and bridge the gaps in current VRE surveillance. Methods The VRE reservoir was investigated using stool samples from 268 inpatients. Characterization of isolated VRE stains consisted of BD Phoenix system, genotypic identification, glycopeptide and quinupristin–dalfopristin (Q–D) resistance probing, virulence gene (esp, hyl, efaA, asa1, gelE, cpd) detection and MLVA. Biofilm formation was evaluated by the microtiter plate method. Results VRE carriage prevalence among at-risk patients was 28.7%. All VRE strains were vanA positive multidrug-resistant Enterococcus faecium (VRfm), harboring ermB-1 (38.9%), esp (84%), efaA (71.2%), hyl (54.5%), asa1 (23.4%), gelE and cpd (11.6%) each. Ability of biofilm production was detected in 20.8%. Genetic relatedness of the isolates revealed 13 clusters, heterogeneous picture and 25 unique MTs profiles. Conclusion The obtained prevalence of VRE intestinal carriage among high-risk inpatients in Serbia is higher than the European average, with high percentage of multidrug resistance. The emergence of resistance to Q–D is of particular concern. Close monitoring of pattern of resistance and strict adherence to specific guidelines are urgently needed in Serbia.

Published
2021
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15. Predictors of Vancomycin-Resistant Enterococcus spp. Intestinal Carriage among High-Risk Patients in University Hospitals in Serbia

Author

Ana Janjusevic, Ivana Cirkovic, Rajna Minic, Goran Stevanovic, Ivan Soldatovic, Biljana Mihaljevic, Ana Vidovic, and Ljiljana Markovic Denic

Subjects
antibiotic-resistance epidemiology, VRE carriage, risk factors, at-risk inpatients, logistic regression, Serbia, Therapeutics. Pharmacology, RM1-950
Abstract

The predictors of intestinal carriage of vancomycin-resistant Enterococcus spp. (VRE) among high-risk patients in the counties of the Southeast Europe Region are insufficiently investigated, yet they could be of key importance in infection control. The aim of the study was to identify risk factors associated with fecal VRE colonization among high-risk inpatients in university hospitals in Serbia. The study comprised 268 inpatients from three university hospitals. Data on patient demographics and clinical characteristics, length of hospital stay, therapy, and procedures were obtained from medical records. Chi-squared tests and univariate and multivariate logistic regressions were performed. Compared to the hemodialysis departments, stay in the geriatric departments, ICUs, and haemato-oncology departments increased the risk for VRE colonization 7.6, 5.4, and 5.5 times, respectively. Compared to inpatients who were hospitalized 48 h before stool sampling for VRE isolation, inpatients hospitalized 3–7, 8–15, and longer than 16 days before sampling had 5.0-, 4.7-, and 6.6-fold higher risk for VRE colonization, respectively. The use of cephalosporins and fluoroquinolones increased the risk for VRE colonization by 2.2 and 1.9 times, respectively. The age ≥ 65 years increased the risk for VRE colonization 2.3 times. In comparison to the University Clinical Centre of Serbia, the hospital stays at Zemun and Zvezdara University Medical Centres were identified as a protector factors. The obtained results could be valuable in predicting the fecal VRE colonization status at patient admission and consequent implementation of infection control measures targeting at-risk inpatients where VRE screening is not routinely performed.

Published
2022
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