Contribution of Spores to the Ability of Clostridium difficile To Adhere to Surfaces

Clostridium difficile is the commonest cause of hospital-acquired infection in the United Kingdom. We characterized the abilities of 21 clinical isolates to form spores; to adhere to inorganic and organic surfaces, including stainless steel and human adenocarcinoma cells; and to germinate. The composition of culture media had a significant effect on spore formation, as significantly more spores were produced in brain heart infusion broth (Student''s t test; P = 0.018). The spore surface relative hydrophobicity (RH) varied markedly (14 to 77%) and was correlated with the ability to adhere to stainless steel. We observed no correlation between the ribotype and the ability to adhere to steel. When the binding of hydrophobic (DS1813; ribotype 027; RH, 77%) and hydrophilic (DS1748; ribotype 002; RH, 14%) spores to human gut epithelial cells at different stages of cell development was examined, DS1813 spores adhered more strongly, suggesting the presence of surface properties that aid attachment to human cells. Electron microscopy studies revealed the presence of an exosporium surrounding DS1813 spores that was absent from spores of DS1748. Finally, the ability of spores to germinate was found to be strain and medium dependent. While the significance of these findings to the disease process has yet to be determined, this study has highlighted the importance of analyzing multiple isolates when attempting to characterize the behavior of a bacterial species.     

Natural Dissemination of Bacillus anthracis Spores in Northern Canada

Soil samples were collected from around fresh and year-old bison carcasses and areas not associated with known carcasses in Wood Buffalo National Park during an active anthrax outbreak in the summer of 2001. Sample selection with a grid provided the most complete coverage of a site. Soil samples were screened for viable Bacillus anthracis spores via selective culture, phenotypic analysis, and PCR. Bacillus anthracis spores were isolated from 28.4% of the samples. The highest concentrations of B. anthracis spores were found directly adjacent to fresh carcasses and invariably corresponded to locations where the soil had been saturated with body fluids escaping the carcass through either natural body orifices or holes torn by scavengers. The majority of positive samples were found within 2 m of both year-old and fresh carcasses and probably originated from scavengers churning up and spreading the body fluid-saturated soil as they fed. Trails of lesser contamination radiating from the carcasses probably resulted from spore dissemination through adhesion to scavengers and through larger scavengers dragging away disarticulated limbs. Comparison of samples from minimally scavenged and fully necropsied carcass sites revealed no statistically significant difference in the level of B. anthracis spore contamination. Therefore, the immediate area around a suspected anthrax carcass should be considered substantially contaminated regardless of the condition of the carcass.     

Fate and Dissemination of Bacillus subtilis Spores in a Murine Model

Bacterial spores are being consumed as probiotics, although little is known about their efficacy or mode of action. As a first step in characterizing spore probiotics, we have studied the persistence and dissemination of Bacillus subtilis spores given orally to mice. Our results have shown that spores do not appear to disseminate across the mucosal surfaces. However, we found that the number of spores excreted in the feces of mice was, in some experiments, larger than the original inoculum. This was an intriguing result and might be explained by germination of a proportion of the spore inoculum in the intestinal tract, followed by limited rounds of cell growth and then sporulation again. This result raises the interesting question of whether it is the spore or the germinated spore that contributes to the probiotic effect of bacterial spores.     

Characterizing the Transmission Potential of Zoonotic Infections from Minor Outbreaks

The transmission potential of a novel infection depends on both the inherent transmissibility of a pathogen, and the level of susceptibility in the host population. However, distinguishing between these pathogen- and population-specific properties typically requires detailed serological studies, which are rarely available in the early stages of an outbreak. Using a simple transmission model that incorporates age-stratified social mixing patterns, we present a novel method for characterizing the transmission potential of subcritical infections, which have effective reproduction number R<1, from readily available data on the size of outbreaks. We show that the model can identify the extent to which outbreaks are driven by inherent pathogen transmissibility and pre-existing population immunity, and can generate unbiased estimates of the effective reproduction number. Applying the method to real-life infections, we obtained accurate estimates for the degree of age-specific immunity against monkeypox, influenza A(H5N1) and A(H7N9), and refined existing estimates of the reproduction number. Our results also suggest minimal pre-existing immunity to MERS-CoV in humans. The approach we describe can therefore provide crucial information about novel infections before serological surveys and other detailed analyses are available. The methods would also be applicable to data stratified by factors such as profession or location, which would make it possible to measure the transmission potential of emerging infections in a wide range of settings.     

Validation of a Nylon-Flocked-Swab Protocol for Efficient Recovery of Bacterial Spores from Smooth and Rough Surfaces

In order to meet planetary-protection requirements, culturable bacterial spore loads are measured representatively for the total microbial contamination of spacecraft. However, the National Aeronautics and Space Administration''s (NASA''s) cotton swab protocols for spore load determination have not changed for decades. To determine whether a more efficient alternative was available, a novel swab was evaluated for recovery of different Bacillus atrophaeus spore concentrations on stainless steel and other surfaces. Two protocols for the nylon-flocked swab (NFS) were validated and compared to the present NASA standard protocol. The results indicate that the novel swab protocols recover 3- to 4-fold more (45.4% and 49.0% recovery efficiency) B. atrophaeus spores than the NASA standard method (13.2%). Moreover, the nylon-flocked-swab protocols were superior in recovery efficiency for spores of seven different Bacillus species, including Bacillus anthracis Sterne (recovery efficiency, 20%). The recovery efficiencies for B. atrophaeus spores from different surfaces showed a variation from 5.9 to 62.0%, depending on the roughness of the surface analyzed. Direct inoculation of the swab resulted in a recovery rate of about 80%, consistent with the results of scanning electron micrographs that allowed detailed comparisons of the two swab types. The results of this investigation will significantly contribute to the cleanliness control of future life detection missions and will provide significant improvement in detection of B. anthracis contamination for law enforcement and security efforts.The recent discovery of liquid water on Mars has sparked debate about the possibility of extraterrestrial life (37). Consequently, highly sensitive biosensors will be deployed onboard spacecraft like the Mars Science Laboratory (MSL), using technologies such as gas chromatographical analysis to search for the smallest traces of life (http://mars.jpl.nasa.gov/msl/mission/). Contamination of equipment by terrestrial microorganisms resulting from a lack of spacecraft cleanliness could significantly compromise the integrity of life detection missions and result in falsely positive extraterrestrial life signals. The prevention of this so-called “forward contamination” is one major goal of American and European space agencies'' planetary-protection efforts. Regular determination of a spacecraft''s bioload and the mission components throughout assembly are mandatory for detecting unacceptably high contamination that exceeds levels set by the United Nations treaty (Outer Space Treaty [11]).Modern spacecraft hardware is very susceptible to standard heat sterilization protocols, so baking the entire spacecraft, such as the Viking Lander Capsule at 111.7°C ± 1.7°C for 23 to 30 h is no longer feasible (30). Alternative cleaning and sterilization methodologies for spacecraft components prior to assembly (i.e., nonthermal plasma technologies) have been discussed (36). However, after integration, sterile hardware is exposed to a significant risk of contamination during assembly, testing, and launching operations. Because of limited access to integrated spacecraft components, the microbial cleanliness of a spacecraft and its surroundings is meticulously maintained through frequent cleaning and sterilization routines. Therefore, the regular and frequent detection of possible contaminants in the assembly environment is more important than ever.To estimate the severity of microbial contamination, the National Aeronautics and Space Administration''s (NASA''s) standard procedure focuses on aerobic, mesophilic spores (26). Briefly, surface samples are taken from spacecraft using moist cotton swabs or wipes. After an extraction procedure, the samples are subjected to a short heat shock (15 min; 80°C) to kill vegetative cells and then pour plated in Trypticase soy agar (TSA) for the enumeration of CFU. This protocol was originally developed for the Viking mission more than 3 decades ago (30) and has remained, for the most part, unchanged.Recent studies have shown that cotton swabs have acceptable recovery efficiencies for Bacillus spores (41.7%) (32) but, due to their organic nature, may raise residue problems on surfaces. Furthermore, their comparatively high DNA content could lead to false positives or inhibition should NASA one day incorporate molecular technologies into their microbial-detection protocols (7).Based on these observations, researchers are beginning to move away from cotton in favor of alternative swabs made from rayon or macrofoam (6, 18). A recent study reported high recovery efficiencies for various vegetative cells from stainless steel surfaces by applying a novel swab with a bulb-shaped head flocked with nylon fibers (12). Patented in 2004, this design facilitates the release of particulates and microbes, resulting in a significantly higher detection rate. The broad applicability of these nylon-flocked swabs (NFS) has been demonstrated by their use in various clinical studies isolating pathogens from medical environments (1, 10, 20).General studies on surface-sampling tools have clearly shown that the swab material and the extraction method are the dominant factors in spore recovery efficiencies (32). Additionally, the properties of the surface to be sampled affect sample recovery (8). For planetary-protection applications, the broad variety of novel materials used in spacecraft construction must be considered. The Mars Exploration Rover mission craft, for example, was composed of at least five kinds of surface materials (http://marsrovers.jpl.nasa.gov/overview). While the cruise stage was constructed primarily of aluminum and the aeroshell consisted of aluminum honeycomb structures, the lander itself was made of titanium and graphite composite (carbon fiber-reinforced plastic [CFRP]). The airbag and the parachutes were made of Vectran and polyester/nylon fabrics. These different materials are quite challenging for sampling tools. Accurate sampling of materials with various surface textures will require planetary-protection programs to introduce novel swab materials.To our knowledge, no investigations have been performed to compare the recovery of spores from different spacecraft surfaces. Previous studies have compared cotton and synthetic sampling materials, but only on stainless steel surfaces (19), and no studies have compared sampling methods on actual spacecraft materials (7).Recently published protocols for spore detection have been based on one specific Bacillus species and/or on one type of surface. Unfortunately, these protocols provide no insight into the effects of varying these factors (4-6, 8, 9, 14, 18), as requested by USP (United States Pharmacopeia) 1223 for validation of alternative microbial methods (3). Some of the aforementioned studies were conducted in response to B. anthracis terrorism incidents in 2001 and used B. atrophaeus as a surrogate. Consequently, information about the actual sampling efficiency of B. anthracis spores is quite limited and may vary significantly from the B. atrophaeus data.In this comprehensive study, we evaluated the novel nylon-flocked swab and a corresponding protocol to recover Bacillus spores from five different spacecraft-related surfaces. It should be noted that although stainless steel served as the standard test surface, it is not a predominant material in spacecraft; however, since the majority of previous (sampling) studies were performed on stainless steel, it represents a universally recognized carrier and also serves as a conservative proxy for the average roughness of the materials used in space science.Our nylon-flocked-swab protocol was validated with respect to accuracy, precision, limit of detection, linearity, and robustness (3). Moreover, its specificity was determined by applying spores of seven different Bacillus species, including the avirulent, attenuated strain Bacillus anthracis Sterne, and by comparing the resulting recovery efficiencies. The results in this communication will significantly contribute to planetary-protection protocols and could also be of high interest for public health issues.     

Evaluation of a Wipe Surface Sample Method for Collection of Bacillus Spores from Nonporous Surfaces

Polyester-rayon blend wipes were evaluated for efficiency of extraction and recovery of powdered Bacillus atrophaeus spores from stainless steel and painted wallboard surfaces. Method limits of detection were also estimated for both surfaces. The observed mean efficiency of polyester-rayon blend wipe recovery from stainless steel was 0.35 with a standard deviation of ±0.12, and for painted wallboard it was 0.29 with a standard deviation of ±0.15. Evaluation of a sonication extraction method for the polyester-rayon blend wipes produced a mean extraction efficiency of 0.93 with a standard deviation of ±0.09. Wipe recovery quantitative limits of detection were estimated at 90 CFU per unit of stainless steel sample area and 105 CFU per unit of painted wallboard sample area. The method recovery efficiency and limits of detection established in this work provide useful guidance for the planning of incident response environmental sampling following the release of a biological agent such as Bacillus anthracis.     

Recovery of Spores from Thermophilic Dairy Bacilli and Effects of Their Surface Characteristics on Attachment to Different Surfaces

Spores from four Geobacillus spp. were isolated from a milk powder manufacturing line in New Zealand. Liquid sporulation media produced spore yields of ~10⁷ spores ml⁻¹; spores were purified using a two-phase system created with polyethylene glycol 4000 and 3 M phosphate buffer. The zeta potentials of the spores from the four isolates ranged from −10 to −20 mV at neutral pH, with an isoelectric point between pH 3 and 4. Through contact angle measurements, spores were found to be hydrophilic and had relative hydrophobicity values of 10 to 40%, as measured by the microbial adhesion to hexadecane assay. The most hydrophilic spore isolate with the smallest negative charge attached in the highest numbers to Thermanox and stainless steel (1 × 10⁴ spores cm⁻²), with fewer spores attaching to glass (3 × 10³ spores cm⁻²). However, spores produced by the other three strains attached in similar numbers (P > 0.05) to all substrata (~1 × 10³ spores cm⁻²), indicating that there was no simple relationship between individual physicochemical interactions and spore adherence. Therefore, surface modifications which limit the attachment of one strain may not be effective for all stains, and control regimens need to be devised with reference to the characteristics of the particular strains of concern.     

Immunoassay Comparison of Haplosporidan Spores from Teredo navalis and Haplosporidium nelsoni Spores from Crassostrea virginica

Spores of a haplosporidan infecting Teredo navalis Linnaeus have been described as morphologically indistinguishable from spores of Haplosporidium nelsoni . To test the hypothesis that these organisms are conspecific, a colloidal gold immunoassay was used to compare antigenic characteristics of the spores from both hosts. Rabbit antibody to formalin-fixed spores from T. navalis was tested against paraffin sections of Crassostrea virginica infected with spores of H. nelsoni and against paraffin sections of infected 7". navalis . Application of primary antibody was followed by addition of affinity purified goat anti-rabbit IgG coaled on 5-nm colloidal gold particles. The reaction was enhanced by precipitation of metallic silver; a positive reaction appeared as a dark brown to black signal at the site of each antigen-antibody complex. Haplosporidium nelsoni spores did not react when assayed with the antibody made to spores from T. navalis . Spores from infected T. navalis tissue reacted positively with rabbit antibody. This result indicates that the spores from the 2 hosts are antigenicaliy distinct and suggests that they are different species.     

Production and Cleaning of Freeze-Etch Replicas which Show Complementary Surfaces of Fractured Fungus Spores and Hyphae

London finder grids (H-2) and 3 mm copper discs were flared on opposite sides by use of a die and punch. The grids were registered on the discs and attached with vaseline. The specimen was squeezed through the grid apertures by the 2 copper discs. The complete sandwich was frozen in freon 22 and placed in a hinged specimen holder which fractured the layer of the specimen between the 2 finder grids. Platinum-carbon and carbon replicas were made immediately after fracturing. After drying the replicas, the vaseline was removed by chloroform, and replicas were cleaned with 70% H₂SO₄ for 1-18 hr at 52 C, followed by 6% commercial sodium hypochlorite (Chlorox) for 1-2 hr at 23-25 C.     

我国转基因Bt抗虫棉的进展分析与生态风险评估

从源头创新、基因转移技术、新品种选育与推广、专利分析四个方面探讨了我国转基因Bt抗虫棉的重大进展。且从靶标昆虫与非目标昆虫两个方面重点对转基因的生态风险进行了综合评价,并根据国内外的研究趋势,提出了加速我国转基因棉研究的对策。     

Experiments with Spores of Aquatic Hyphomycetes: I. Sedimentation, and Impaction on Smooth Surfaces

Techniques are described for the production of heavy concentrationsof aquatic Hyphomycete spores, for estimating the spore concentration,the sedimentation rate of spores and their trapping efficiencyon smooth cylinders. No correlation could be discovered betweenthe rates of sedimentation and spore shape. Trapping experimentsshowed that the trapping efficiency of the tetraradiate sporeswas higher than that of spores of different shape. It is suggestedthat the higher efficiency might be the result of contact ofthe tetraradiate spore at three points on a surface.     

Molecular Method To Assess the Diversity of Burkholderia Species in Environmental Samples

In spite of the importance of many members of the genus Burkholderia in the soil microbial community, no direct method to assess the diversity of this genus has been developed so far. The aim of this work was the development of soil DNA-based PCR-denaturing gradient gel electrophoresis (DGGE), a powerful tool for studying the diversity of microbial communities, for detection and analysis of the Burkholderia diversity in soil samples. Primers specific for the genus Burkholderia were developed based on the 16S rRNA gene sequence and were evaluated in PCRs performed with genomic DNAs from Burkholderia and non-Burkholderia species as the templates. The primer system used exhibited good specificity and sensitivity for the majority of established species of the genus Burkholderia. DGGE analyses of the PCR products obtained showed that there were sufficient differences in migration behavior to distinguish the majority of the 14 Burkholderia species tested. Sequence analysis of amplicons generated with soil DNA exclusively revealed sequences affiliated with sequences of Burkholderia species, demonstrating that the PCR-DGGE method is suitable for studying the diversity of this genus in natural settings. A PCR-DGGE analysis of the Burkholderia communities in two grassland plots revealed differences in diversity mainly between bulk and rhizosphere soil samples; the communities in the latter samples produced more complex patterns.     

Cold Air Plasma To Decontaminate Inanimate Surfaces of the Hospital Environment

The hospital environment harbors bacteria that may cause health care-associated infections. Microorganisms, such as multiresistant bacteria, can spread around the patient''s inanimate environment. Some recently introduced biodecontamination approaches in hospitals have significant limitations due to the toxic nature of the gases and the length of time required for aeration. This study evaluated the in vitro use of cold air plasma as an efficient alternative to traditional methods of biodecontamination of hospital surfaces. Cultures of methicillin-resistant Staphylococcus aureus (MRSA), vancomycin-resistant enterococci (VRE), extended-spectrum-β-lactamase (ESBL)-producing Escherichia coli, and Acinetobacter baumannii were applied to different materials similar to those found in the hospital environment. Artificially contaminated sections of marmoleum, mattress, polypropylene, powder-coated mild steel, and stainless steel were then exposed to a cold air pressure plasma single jet for 30 s, 60 s, and 90 s, operating at approximately 25 W and 12 liters/min flow rate. Direct plasma exposure successfully reduced the bacterial load by log 3 for MRSA, log 2.7 for VRE, log 2 for ESBL-producing E. coli, and log 1.7 for A. baumannii. The present report confirms the efficient antibacterial activity of a cold air plasma single-jet plume on nosocomial bacterially contaminated surfaces over a short period of time and highlights its potential for routine biodecontamination in the clinical environment.     

Mapping the Risk of Soil-Transmitted Helminthic Infections in the Philippines

BackgroundIn order to increase the efficient allocation of soil-transmitted helminth (STH) disease control resources in the Philippines, we aimed to describe for the first time the spatial variation in the prevalence of A. lumbricoides, T. trichiura and hookworm across the country, quantify the association between the physical environment and spatial variation of STH infection and develop predictive risk maps for each infection.Conclusions/SignificanceThis analysis revealed significant spatial variation in STH infection prevalence within provinces of the Philippines. This suggests that a spatially targeted approach to STH interventions, including mass drug administration, is warranted. When financially possible, additional STH surveys should be prioritized to high-risk areas identified by our study in Luzon.