Roger G. Kern
California Institute of Technology
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Featured researches published by Roger G. Kern.
Journal of Microbiological Methods | 2003
Kasthuri Venkateswaran; Noriaki Hattori; Myron T. La Duc; Roger G. Kern
A new firefly luciferase bioluminescence assay method that differentiates free extracellular ATP (dead cells, etc.) from intracellular ATP (viable microbes) was used to determine the viable microbial cleanliness of various clean-room facilities. For comparison, samples were taken from both clean-rooms, where the air was filtered to remove particles >0.5 microm, and ordinary rooms with unfiltered air. The intracellular ATP was determined after enzymatically degrading the samples free ATP. Also for comparison, cultivable microbial populations were counted on nutrient-rich trypticase soy agar (TSA) plates. Both the cultivable and ATP-based determinations indicate that the microbial burden was lower in clean-room facilities than in ordinary rooms. However, there was no direct correlation between the two sets of measurements because the two assays measured very different populations. A large fraction of the samples yielded no colony formers on TSA, but were positive for intracellular ATP. Subsequently, genomic DNA was isolated directly from selected samples and 16S rDNA fragments were cloned and sequenced, identifying nearest neighbors, many of which are known to be noncultivable in the media employed. It was concluded that viable microbial contamination can be reliably monitored by measurement of intracellular ATP, and that this method may be considered superior to cultivable colony counts due to its speed and its ability to report the presence of viable but noncultivable organisms. When the detection of nonviable microbes is of interest, the ATP assay can be supplemented with DNA analysis.
Systematic and Applied Microbiology | 2001
Kasthuri Venkateswaran; Masataka Satomi; Shirley Y. Chung; Roger G. Kern; Robert Koukol; Cecilia Basic; David White
In ongoing investigations to map and archive the microbial footprints in various components of the spacecraft and its accessories, we have examined the microbial populations of the Jet Propulsion Laboratorys Spacecraft Assembly Facility (JPL-SAF). Witness plates made up of spacecraft materials, some painted with spacecraft qualified paints, were exposed for approximately 7 to 9 months at JPL-SAF and examined the particulate materials collected for the incidence of total cultivable aerobic heterotrophs and heat-tolerant (80 degrees C for 15-min.) spore-formers. The results showed that the witness plates coated with spacecraft qualified paints attracted more dust particles than the non-coated stainless steel witness plates. Among the four paints tested, witness plates coated with NS43G accumulated the highest number of particles, and hence attracted more cultivable microbes. The conventional microbiological examination revealed that the JPL-SAF harbors mainly Gram-positive microbes and mostly spore-forming Bacillus species. Most of the isolated microbes were heat resistant to 80 degrees C and proliferate at 60 degrees C. The phylogenetic relationships among 23 cultivable heat-tolerant microbes were examined using a battery of morphological, physiological, molecular and chemotaxonomic characterizations. By 16S rDNA sequence analysis, the isolates fell into seven clades: Bacillus licheniformis, B. pumilus, B. cereus, B. circulans, Staphylococcus capitis, Planococcus sp. and Micrococcus lylae. In contrast to the cultivable approach, direct DNA isolation, cloning and 16S rDNA sequencing analysis revealed equal representation of both Gram-positive and Gram-negative microorganisms.
Microbial Ecology | 2004
M. T. La Duc; Roger G. Kern; Kasthuri Venkateswaran
Rapid microbial monitoring technologies are invaluable in assessing contamination of spacecraft and associated environments. Universal and widespread elements of microbial structure and chemistry are logical targets for assessing microbial burden. Several biomarkers such as ATP, LPS, and DNA (ribosomal or spore-specific), were targeted to quantify either total bioburden or specific types of microbial contamination. The findings of these assays were compared with conventional, culture-dependent methods. This review evaluates the applicability and efficacy of some of these methods in monitoring the microbial burden of spacecraft and associated environments. Samples were collected from the surfaces of spacecraft, from surfaces of assembly facilities, and from drinking water reservoirs aboard the International Space Station (ISS). Culture-dependent techniques found species of Bacillus to be dominant on these surfaces. In contrast, rapid, culture-independent techniques revealed the presence of many Gram-positive and Gram-negative microorganisms, as well as actinomycetes and fungi. These included both cultivable and noncultivable microbes, findings further confirmed by DNA-based microbial detection techniques. Although the ISS drinking water was devoid of cultivable microbes, molecular-based techniques retrieved DNA sequences of numerous opportunistic pathogens. Each of the methods tested in this study has its advantages, and by coupling two or more of these techniques even more reliable information as to microbial burden is rapidly obtained.
international conference on evolvable systems | 2000
Kasthuri Venkateswaran; C. Echeverria; A. Vu; M. Musick; Shirley Y. Chung; Robert Koukol; Roger G. Kern; D. C. White; M. Satomi
Microbial biofilms representing both Gram-positive and Gram-negative bacteria were artificially coated onto aluminum metal surfaces that are chiefly used in building spacecraft.
Environmental Microbiology | 2003
Myron T. La Duc; Wayne Nicholson; Roger G. Kern; Kasthuri Venkateswaran
Astrobiology | 2005
Michael Kempf; Fei Chen; Roger G. Kern; Kasthuri Venkateswaran
International Journal of Systematic and Evolutionary Microbiology | 2003
Kasthuri Venkateswaran; Michael Kempf; Fei Chen; Masataka Satomi; Wayne Nicholson; Roger G. Kern
Astrobiology | 2004
Kasthuri Venkateswaran; Shirley Y. Chung; Judith Allton; Roger G. Kern
Astrobiology | 2005
Andrew C. Schuerger; Jeffrey T. Richards; Paul E. Hintze; Roger G. Kern
Archive | 1996
David A. Kidwell; Gil F. Richards; Roger G. Kern; Frederick W. Mintz