Your search keyword '"Nelis, H."' showing total 15 results

1. Procaine Induces Cytokinesis in Horse Oocytes via a pH-Dependent Mechanism.

Author

Leemans B, Gadella BM, Stout TA, Heras S, Smits K, Ferrer-Buitrago M, Claes E, Heindryckx B, De Vos WH, Nelis H, Hoogewijs M, and Van Soom A

Subjects

Animals, Chromatin metabolism, Female, Fertilization in Vitro veterinary, Horses, Hydrogen-Ion Concentration, Male, Oocytes metabolism, Sperm Injections, Intracytoplasmic veterinary, Spermatozoa physiology, Cytokinesis drug effects, Oocytes drug effects, Procaine pharmacology, Sperm-Ovum Interactions drug effects, Spermatozoa drug effects

Abstract

Coincubating equine gametes in the presence of procaine has been reported to facilitate in vitro fertilization, with cleavage rates exceeding 60%. We report that while procaine does trigger sperm hyperactivation, it independently induces cleavage of equine oocytes. First, we found that procaine (1-5 mM) did not facilitate stallion sperm penetration of equine oocytes but instead induced sperm-independent oocyte cytokinesis in the absence of the second polar body extrusion. Indeed, 56 ± 4% of oocytes cleaved within 2.5 days of exposure to 2.5 mM procaine regardless of sperm presence. However, the cleaved oocytes did not develop beyond 8 to 16 cells, and the daughter cells either lacked nuclei or contained aberrant, condensed DNA fragments. By contrast, intracytoplasmic sperm injection (ICSI) was followed by second polar body extrusion and formation of normal blastocysts. Moreover, neither the calcium oscillations detectable using fura-2 AM staining nor the cortical granule reaction visualized by LCA-FITC staining, after oocyte activation induced by ICSI or ionomycin treatment, were detected after exposing oocytes to 2.5 mM procaine. Instead, procaine initiated an ooplasmic alkalinization, detectable by BCECF-AM staining that was not observed after other treatments. This alkalinization was followed, after an additional 18 h of incubation, by cortical F-actin depolymerization, as demonstrated by reduced actin phalloidin-FITC staining intensity, that resembled preparation for cytokinesis in ICSI-fertilized zygotes. Overall, we conclude that procaine induces cytokinesis in equine oocytes accompanied by aberrant chromatin condensation and division; this explains why embryos produced after exposing equine oocytes to procaine fail to develop beyond the 8- to 16-cell stage., (© 2015 by the Society for the Study of Reproduction, Inc.)

Published

2015

2. Oviduct binding and elevated environmental ph induce protein tyrosine phosphorylation in stallion spermatozoa.

Author

Leemans B, Gadella BM, Sostaric E, Nelis H, Stout TA, Hoogewijs M, and Van Soom A

Subjects

Animals, Female, Fertilization physiology, Horses, Male, Phosphorylation, Protein-Tyrosine Kinases metabolism, Oviducts metabolism, Sperm Capacitation physiology, Spermatozoa metabolism, Tyrosine metabolism

Abstract

Sperm-oviduct binding is an essential step in the capacitation process preparing the sperm for fertilization in several mammalian species. In many species, capacitation can be induced in vitro by exposing spermatozoa to bicarbonate, Ca(2+), and albumin; however, these conditions are insufficient in the horse. We hypothesized that binding to the oviduct epithelium is an essential requirement for the induction of capacitation in stallion spermatozoa. Sperm-oviduct binding was established by coincubating equine oviduct explants for 2 h with stallion spermatozoa (2 × 10(6) spermatozoa/ml), during which it transpired that the highest density (per mm(2)) of oviduct-bound spermatozoa was achieved under noncapacitating conditions. In subsequent experiments, sperm-oviduct incubations were performed for 6 h under noncapacitating versus capacitating conditions. The oviduct-bound spermatozoa showed a time-dependent protein tyrosine phosphorylation response, which was not observed in unbound spermatozoa or spermatozoa incubated in oviduct explant conditioned medium. Both oviduct-bound and unbound sperm remained motile with intact plasma membrane and acrosome. Since protein tyrosine phosphorylation can be induced in equine spermatozoa by media with high pH, the intracellular pH (pHi) of oviduct explant cells and bound spermatozoa was monitored fluorometrically after staining with BCECF-AM dye. The epithelial secretory cells contained large, alkaline vesicles. Moreover, oviduct-bound spermatozoa showed a gradual increase in pHi, presumably due to an alkaline local microenvironment created by the secretory epithelial cells, given that unbound spermatozoa did not show pHi changes. Thus, sperm-oviduct interaction appears to facilitate equine sperm capacitation by creating an alkaline local environment that triggers intracellular protein tyrosine phosphorylation in bound sperm., (© 2014 by the Society for the Study of Reproduction, Inc.)

Published

2014

3. Biofilm inhibitory and eradicating activity of wound care products against Staphylococcus aureus and Staphylococcus epidermidis biofilms in an in vitro chronic wound model.

Author

Brackman G, De Meyer L, Nelis HJ, and Coenye T

Subjects

Bacterial Load, Bandages, Humans, Models, Biological, Staphylococcal Infections microbiology, Wound Healing, Wound Infection microbiology, Biofilms, Staphylococcal Infections therapy, Staphylococcus aureus, Staphylococcus epidermidis, Wound Infection therapy

Abstract

Aims: Although several factors contribute to wound healing, bacterial infections and the presence of biofilm can significantly affect healing. Despite that this clearly indicates that therapies should address biofilm in wounds, only few wound care products have been evaluated for their antibiofilm effect. For this reason, we developed a rapid quantification approach to investigate the efficacy of wound care products on wounds infected with Staphylococcus spp., Methods and Results: An in vitro chronic wound infection model was used in which a fluorescent Staph. aureus strain was used to allow the rapid quantification of the bacterial burden after treatment. A good correlation was observed between the fluorescence signal and the bacterial counts. When evaluated in this model, several commonly used wound dressings and wound care products inhibited biofilm formation resulting in a decrease between one and seven log CFU per biofilm compared with biofilm formed in the absence of products. In contrast, most dressings only moderately affected mature biofilms., Conclusion: Our model allowed the rapid quantification of the bacterial burden after treatment. However, the efficacy of treatment varied between the different types of dressings and/or wound care products., Significance and Impact of the Study: Our model can be used to compare the efficacy of wound care products to inhibit biofilm formation and/or eradicate mature biofilms. In addition, the results indicate that treatment of infected wounds should be started as soon as possible and that novel products with more potent antibiofilm activity are needed., (© 2013 The Society for Applied Microbiology.)

Published

2013

4. Quality control of Saccharomyces boulardii- a response to the Letter of Honraet and Delcour (2011).

Author

Coenye T and Nelis HJ

Subjects

Animals, Clostridium Infections prevention & control, Germ-Free Life physiology, Probiotics pharmacology, Probiotics standards, Saccharomyces physiology, Saccharomyces cerevisiae growth & development, Salmonella Infections prevention & control

Published

2011

5. Quality control of fifteen probiotic products containing Saccharomyces boulardii.

Author

Vanhee LM, Goemé F, Nelis HJ, and Coenye T

Subjects

Colony Count, Microbial, Image Cytometry, Microbial Viability, Microsatellite Repeats genetics, Quality Control, Saccharomyces genetics, Stomach microbiology, Time Factors, Probiotics standards, Saccharomyces physiology

Abstract

Aims: The yeast Saccharomyces boulardii is used as a probiotic for the prevention and treatment of diarrhoea. In this study, the quality of 15 probiotic products containing S. boulardii was verified., Methods and Results: Using microsatellite typing, the identity of all Saccharomyces strains in the products was confirmed as S. boulardii. Additionally, solid-phase cytometry (SPC) and a plate method were used to enumerate S. boulardii cells. SPC was not only able to produce results more rapidly than plating (4h compared to 48h) but the cell counts obtained with SPC were significantly higher than the plate counts. Finally, we found that <1% of the S. boulardii cells survived 120min in gastric conditions and storage for 3months at 40°C with 75% relative humidity., Conclusions: We developed a SPC method for the quantification of viable S. boulardii cells in probiotics. Additionally, we demonstrated that gastric conditions and storage have a marked effect on the viability of the yeast cells., Significance and Impact of the Study:   To our knowledge, this is the first time SPC is used for the quality control of probiotics with S. boulardii. Additionally, we demonstrated the need for gastric protection and accurate storage., (© 2010 The Authors. Journal of Applied Microbiology © 2010 The Society for Applied Microbiology.)

Published

2010

6. Comparison of solid-phase cytometry and the plate count method for the evaluation of the survival of bacteria in pharmaceutical oils.

Author

De Prijck K, Peeters E, and Nelis HJ

Subjects

Bacteria isolation & purification, Colony Count, Microbial methods, Laser Scanning Cytometry methods, Anti-Bacterial Agents pharmacology, Bacteria drug effects, Microbial Viability drug effects, Plant Oils pharmacology

Abstract

Aim: To compare the survival of four bacterial strains (Escherichia coli, Proteus mirabilis, Staphylococcus aureus, Pseudomonas aeruginosa) in pharmaceutical oils, including jojoba oil/tea tree oil, carbol oil, jojoba oil and sesame oil., Methods and Results: Oils were spiked with the test bacteria in a concentration of 10(4) CFU ml(-1). Bacteria were extracted from oils with phosphate-buffered saline containing 0.5% Tween 20. Aliquots of the pooled water layers were analysed by solid-phase cytometry and plate counting. Plate counts dropped to zero for all test strains exposed for 24 h to three of the four oils. In contrast, significant numbers of viable cells were still detected by SPC, except in the jojoba oil/tea tree oil mixture and partly in sesame oil., Conclusions: Exposure of bacteria for 24 h to the two oils containing an antimicrobial led to a loss of their culturability but not necessarily of their viability. The antibacterial activity of the jojoba oil/tea tree oil mixture supersedes that of carbol oil., Significance and Impact of the Study: These in vitro data suggest that the jojoba oil/tea tree oil mixture more than carbol oil inhibits bacterial proliferation when used for intermittent self-catherization.

Published

2008

7. Microbiological challenge of four protective devices for the reconstitution of cytotoxic agents.

Author

De Prijck K, D'Haese E, Vandenbroucke J, Coucke W, Robays H, and Nelis HJ

Subjects

Bacteria drug effects, Disinfectants pharmacology, Cytotoxins, Disinfection methods, Equipment Contamination statistics & numerical data, Protective Devices microbiology

Abstract

Aims: To evaluate the susceptibility to microbial contamination that occurs during simulated handling of protective devices for the preparation of cytotoxic drug solutions., Methods and Results: Four devices, i.e. Chemoprotect spike, Clave connector, PhaSeal and Securmix were challenged with low and high inocula of micro-organisms. The cells, transferred to the connected vials during repeated manipulations of the devices were counted by means of solid-phase cytometry. Of the four devices, PhaSeal afforded the lowest transfer of micro-organisms. Secondly, the efficiency of procedures for the disinfection of an artificially contaminated rubber stopper was compared prior to connection of the vial to the PhaSeal device. Spraying or swabbing alone was inadequate, as opposed to a combination of spraying [0.5% or 2.0% (w/v) chlorhexidine in isopropanol] and swabbing [70% (v/v) isopropanol]., Conclusions: Although Phaseal afforded the lowest transfer of micro-organisms, adequate disinfection of the vial prior to connection remains required., Significance and Impact of the Study: Unlike aspects of operator protection, which are well documented, the microbiological safety of protective devices for the preparation of cytotoxic drugs has not been addressed in the literature. This study estimates the susceptibility to microbial contamination during handling of four commonly used devices.

Published

2008

8. Use of the modified Robbins device to study the in vitro biofilm removal efficacy of NitrAdine, a novel disinfecting formula for the maintenance of oral medical devices.

Author

Coenye T, De Prijck K, De Wever B, and Nelis HJ

Subjects

Candida albicans drug effects, Disinfection methods, Humans, Microbial Sensitivity Tests methods, Plankton drug effects, Biofilms drug effects, Denture Cleansers pharmacology, Disinfectants pharmacology, Oral Hygiene

Abstract

Aims: To evaluate the use of the modified Robbins device (MRD) to test disinfection strategies against biofilms that form on oral medical devices and to test the biofilm removal efficacy of NitrAdine, a disinfectant for the maintenance of oral medical devices., Methods and Results: Biofilms were grown on discs using the MRD and biofilms formed in this system were used to evaluate the efficacy of NitrAdine and to determine the optimal disinfection conditions. Our data indicate that the use of the MRD allows for the rapid and reproducible formation of high-density biofilms. Determination of the efficacy of NitrAdine revealed high activity against biofilms tested (e.g. >3 log reduction for Candida albicans and Staphylococcus aureus) and allowed the determination of the optimal conditions for its use., Conclusion: The high reproducibility and flexibility of the MRD make it an excellent candidate for standardized testing of disinfectants aimed at reducing biofilms on oral medical devices. Using this system, we were able to demonstrate that NitrAdine exhibits high activity against biofilms formed by the micro-organisms tested., Significance and Impact of the Study: Our data suggest that our procedure is appropriate for standardized testing of disinfectants aimed at reducing biofilms on oral medical devices.

Published

2008

9. Persistence of Campylobacter jejuni on surfaces in a processing environment and on cutting boards.

Author

Cools I, Uyttendaele M, Cerpentier J, D'Haese E, Nelis HJ, and Debevere J

Subjects

Animals, Campylobacter jejuni isolation & purification, Colony Count, Microbial, Environmental Microbiology, Time Factors, Campylobacter jejuni growth & development, Equipment Contamination, Food Handling, Poultry

Abstract

Aims: The objectives of the study were to determine the spread and persistence of Campylobacter in a poultry processing plant and to provide a quantitative estimate of the survival of Campylobacter jejuni on the surface of a cutting board., Methods and Results: Several contact surfaces in a poultry processing plant were sampled before the start of processing, after 30 min and after 120 min. Next, the survival of four C. jejuni strains was studied on a beech and polypropylene cutting board during 120 min., Conclusions: A rapid introduction and spread of Campylobacter in a well cleaned processing plant as well as a significant survival in time on the example of a cutting board is shown., Significance and Impact of the Study: The need to prevent cross-contamination in the food processing and preparation area and the importance of an integrated approach throughout the whole food chain to control transmission of Campylobacter is highlighted.

Published

2005

10. Burkholderia cepacia complex genomovars: utilization of carbon sources, susceptibility to antimicrobial agents and growth on selective media.

Author

Vermis K, Vandamme PA, and Nelis HJ

Subjects

Burkholderia cepacia drug effects, Burkholderia cepacia genetics, Burkholderia cepacia growth & development, Carbon metabolism, Culture Media, Genotype, Microbial Sensitivity Tests, Phenotype, Burkholderia cepacia classification

Abstract

Aims: To investigate the relationship between genomovar status and carbon source utilization, antibiotic susceptibility and growth ability on selective media of 142 clinical and environmental Burkholderia cepacia complex (Bcc) isolates belonging to all nine genomovars., Methods and Results: Carbon source utilization and growth on selective media were tested by agar plate multipoint inoculation. Antimicrobial minimum inhibitory concentration (MIC) values were determined by agar dilution. Of all carbon sources, l-arabinose was most frequently utilized, supporting growth of 90% of all isolates. Burkholderia cepacia genomovar VI failed to utilize azelaic acid, penicillin G, phtalate, salicin and tryptamine. Overall, B. vietnamiensis and B. anthina were most susceptible and B. cepacia genomovar VI most resistant to antimicrobial agents. Burkholderia cepacia selective agar (BCSA) and the Mast B. cepacia medium supported growth of Bcc isolates most efficiently., Conclusions: This study demonstrates phenotypic heterogeneity within the Bcc. Some trends can be observed at the genomovar level, but only B. cepacia genomovar VI could be differentiated unambiguously on the basis of its inability to grow on PCAT., Significance and Impact of the Study: This work provides an update on some differential phenotypic characteristics of all nine Bcc genomovars.

Published

2003

11. Survival of Campylobacter jejuni strains of different origin in drinking water.

Author

Cools I, Uyttendaele M, Caro C, D'Haese E, Nelis HJ, and Debevere J

Subjects

Animals, Bacteriological Techniques methods, Colony Count, Microbial, Culture Media, Humans, Poultry microbiology, Reproducibility of Results, Temperature, Campylobacter jejuni growth & development, Water Microbiology, Water Supply

Abstract

Aims: The aim of the study was to measure the survival of 19 Campylobacter jejuni strains of different origins, including two reference strains, four poultry-derived isolates, nine human isolates and four water isolates, in sterilized drinking water., Methods and Results: Pure cultures of 19 C. jejuni strains were inoculated in sterile drinking water and incubated at 4 degrees C for 64 days. Survival was determined by culturability on both selective (Karmali agar) and non-selective [Columbia blood agar (CBA)] media. Culturability was shown to be strain and origin-dependent. Campylobacter jejuni showed prolonged survival on a non-selective than on a selective medium., Conclusions: The origin of the strain is a determining factor for the survival of C. jejuni in drinking water at 4 degrees C. Poultry isolates showed a prolonged survival, which could be an indication that these strains could play an important role in the transmission of campylobacteriosis through water. In addition, culture conditions are an important factor for evaluating the survival of C. jejuni in drinking water at 4 degrees C. The non-selective agar (CBA) allowed growth of C. jejuni over a longer period of time than the selective agar (Karmali). Furthermore, an enrichment broth (Bolton) allowed the recovery of all 19 C. jejuni strains during the 64 days of incubation at 4 degrees C., Significance and Impact of the Study: This study highlighted differences in culturability depending on culture conditions and on strain origin.

Published

2003

12. Colonization of a voice prosthesis by Cryptococcus neoformans.

Author

Bauters TG, Moerman M, Pini G, Vermeersch H, and Nelis HJ

Subjects

Animals, Carcinoma, Columbidae microbiology, Cryptococcus neoformans classification, Cryptococcus neoformans isolation & purification, Feces microbiology, Glottis, Humans, Laryngeal Neoplasms rehabilitation, Laryngeal Neoplasms surgery, Laryngectomy, Male, Cryptococcus neoformans growth & development, Larynx, Artificial microbiology

Abstract

Tracheoesophageal voice prostheses in laryngectomized patients commonly deteriorate due to the presence of yeasts, particularly Candida species. We describe the first case of colonization of such a device by Cryptococcus neoformans in a patient with a history of glottic carcinoma. The isolate showed an identical genomic pattern with C. neoformans from pigeon excreta in the patient's environment.

Published

2001

13. Effect of antibiotics on viability staining of Escherichia coli in solid phase cytometry.

Author

D'Haese E and Nelis HJ

Subjects

Colistin pharmacology, Dose-Response Relationship, Drug, Escherichia coli physiology, Flow Cytometry methods, Fluorescent Dyes, Anti-Bacterial Agents pharmacology, Escherichia coli drug effects, Microbial Sensitivity Tests methods

Abstract

Solid phase cytometry (SPC) has been investigated as a tool to assess the effect of antibiotics on the viability of Escherichia coli. After exposure of the cells to the antibiotic, they are retained on a polyester membrane filter and labelled using a fluorescein derivative as a substrate for intracellular esterases. The number of fluorescent bacteria is automatically counted in an Ar laser scanning device. In the presence of nutrients, all antibiotics tested in concentrations exceeding the MIC inhibited the multiplication of cells but not the labelling per se. However, when no nutrients were added, the cells did not multiply, and inhibition of the fluorescent staining was only observed for membrane permeabilizing antibiotics, even at sub-MIC concentrations. The selective detection by SPC of membrane-permeabilizing antibiotics corroborates the requirement of membrane integrity for viability labelling of bacteria. This selectivity has been exploited to develop a method for the detection of colistin residues in milk.

Published

2000

14. A 210-min solid phase cytometry test for the enumeration of Escherichia coli in drinking water.

Author

Van Poucke SO and Nelis HJ

Subjects

Filtration, Fluorometry, Fresh Water microbiology, Glucuronidase analysis, Sensitivity and Specificity, Sewage microbiology, beta-Galactosidase analysis, Colony Count, Microbial methods, Escherichia coli isolation & purification, Water Microbiology

Abstract

A 210-min-test for the enumeration of Escherichia coli in drinking water is described, based on solid phase cytometry (SPC) and a two-step enzymatic procedure for fluorescence labelling of single cells and small microcolonies. The test involves membrane filtration through a 25-mm black polyester filter, induction of beta-glucuronidase in the retained target cells, fluorescence labelling with fluorescein-di-beta-Dglucuronide as an enzyme substrate and laser scanning of the membrane filter. Scan results can be confirmed on-line by epifluorescence microscopy. Application to 149 naturally contaminated and uncontaminated well, tap, out-of-pump centre (distribution), surface and sewage-spiked water samples indicated > or =90% agreement and equivalence with plate count methods, including Chromocult Coliform agar and m FC agar. In 5.4% of all samples examined, SPC detected between 1 and 11 E. coli per 100 ml, while the two plate methods yielded negative results. Cases of a negative SPC result but a positive E. coli count on both reference media were not observed. This test would primarily be useful for 'emergency' monitoring of drinking water when rapid results are crucial.

Published

2000

15. Nonaqueous reversed-phase liquid chromatography and fluorimetry compared for determination of retinol in serum.

Author

Nelis HJ, De Roose J, Vandenbavière H, and De Leenheer AP

Subjects

Chromatography, High Pressure Liquid, Chromatography, Liquid, Fluorometry, Humans, Vitamin A analogs & derivatives, Vitamin A isolation & purification, Vitamin A blood

Abstract

A new assay for retinol in human serum, based on nonaqueous reversed-phase liquid chromatography, is presented. Sample preparation includes addition of the internal standard, retinyl propionate, deproteinization of 100 microL of serum with acetonitrile, and extraction with hexane. The standard curve is linear up to 2 mg/L. The assay is characterized by excellent sensitivity (detection limit, 15 micrograms/L) and good within-run and between-run precision (CVs of 2.6 and 2.7%, respectively), and results compare favorably with those by fluorimetry. We assayed 135 samples from hospitalized patients by both methods. Although the two sets of values correlated well (r = 0.955) the fluorimetric method occasionally suffers from interferences. In practice, fluorimetry proves valuable as a routine method, while liquid chromatography meets the criteria of a potential reference method.

Published

1983