Kristina M. Obom
Johns Hopkins University
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Publication
Featured researches published by Kristina M. Obom.
Journal of Visualized Experiments | 2013
Patrick J. Cummings; Ray Ahmed; Jeffrey A. Durocher; Adam Jessen; Tamar Vardi; Kristina M. Obom
Pyrosequencing is a versatile technique that facilitates microbial genome sequencing that can be used to identify bacterial species, discriminate bacterial strains and detect genetic mutations that confer resistance to anti-microbial agents. The advantages of pyrosequencing for microbiology applications include rapid and reliable high-throughput screening and accurate identification of microbes and microbial genome mutations. Pyrosequencing involves sequencing of DNA by synthesizing the complementary strand a single base at a time, while determining the specific nucleotide being incorporated during the synthesis reaction. The reaction occurs on immobilized single stranded template DNA where the four deoxyribonucleotides (dNTP) are added sequentially and the unincorporated dNTPs are enzymatically degraded before addition of the next dNTP to the synthesis reaction. Detection of the specific base incorporated into the template is monitored by generation of chemiluminescent signals. The order of dNTPs that produce the chemiluminescent signals determines the DNA sequence of the template. The real-time sequencing capability of pyrosequencing technology enables rapid microbial identification in a single assay. In addition, the pyrosequencing instrument, can analyze the full genetic diversity of anti-microbial drug resistance, including typing of SNPs, point mutations, insertions, and deletions, as well as quantification of multiple gene copies that may occur in some anti-microbial resistance patterns.
Journal of Visualized Experiments | 2014
Kristina M. Obom; Patrick J. Cummings; Janelle A. Ciafardoni; Yasunori Hashimura; Daniel Giroux
Recent advances in mammalian, insect, and stem cell cultivation and scale-up have created tremendous opportunities for new therapeutics and personalized medicine innovations. However, translating these advances into therapeutic applications will require in vitro systems that allow for robust, flexible, and cost effective bioreactor systems. There are several bioreactor systems currently utilized in research and commercial settings; however, many of these systems are not optimal for establishing, expanding, and monitoring the growth of different cell types. The culture parameters most challenging to control in these systems include, minimizing hydrodynamic shear, preventing nutrient gradient formation, establishing uniform culture medium aeration, preventing microbial contamination, and monitoring and adjusting culture conditions in real-time. Using a pneumatic single-use bioreactor system, we demonstrate the assembly and operation of this novel bioreactor for mammalian cells grown on micro-carriers. This bioreactor system eliminates many of the challenges associated with currently available systems by minimizing hydrodynamic shear and nutrient gradient formation, and allowing for uniform culture medium aeration. Moreover, the bioreactor’s software allows for remote real-time monitoring and adjusting of the bioreactor run parameters. This bioreactor system also has tremendous potential for scale-up of adherent and suspension mammalian cells for production of a variety therapeutic proteins, monoclonal antibodies, stem cells, biosimilars, and vaccines.
Journal of Visualized Experiments | 2013
Kristina M. Obom; Andrew Magno; Patrick J. Cummings
Fermentation systems are used to provide an optimal growth environment for many different types of cell cultures. The ability afforded by fermentors to carefully control temperature, pH, and dissolved oxygen concentrations in particular makes them essential to efficient large scale growth and expression of fermentation products. This video will briefly describe the advantages of the fermentor over the shake flask. It will also identify key components of a typical benchtop fermentation system and give basic instruction on setup of the vessel and calibration of its probes. The viewer will be familiarized with the sterilization process and shown how to inoculate the growth medium in the vessel with culture. Basic concepts of operation, sampling, and harvesting will also be demonstrated. Simple data analysis and system cleanup will also be discussed.
Journal of Microbiology & Biology Education | 2009
Grace A. Maldarelli; Erica M. Hartmann; Patrick J. Cummings; Robert D. Horner; Kristina M. Obom; Richard Shingles; Rebecca S. Pearlman
Journal of Microbiology & Biology Education | 2007
Kristina M. Obom; Patrick J. Cummings
Archive | 2009
Kristina M. Obom; Gary Brooker; Maria DeBernardi; Patrick J. Cummings
Archive | 2008
Patrick J. Cummings; Kristina M. Obom
Archive | 2008
Patrick J. Cummings; Kristina M. Obom
Archive | 2007
Patrick J. Cummings; Kristina M. Obom
Archive | 2007
Patrick J. Cummings; Kristina M. Obom