Abstract

Purpose and Program Characteristics The purpose of this training program is to provide a curriculum and research environment that will prepare trainees in chemical engineering, chemistry and cell and molecular biology at the predoctoral level for careers in biotechnology. Specifically, this program focuses on research training in areas relevant to the needs of biotechnology, pharmaceutical and chemical companies currently involved in the manufacture of products using biological routes and includes areas such as molecular genetics, fermentation, mammalian cell culture, enzyme technology, bioproduct recovery, combinatorial biocatalysis, combinatorial chemistry. The graduate program includes laboratory and classroom instruction in cell culture techniques (mammalian and bacteria cell culture), protein and enzyme isolation, purification and immobilization, mutagenesis and gene expression, protein and nucleic acid chemistry and biochemistry, and separation and purification methods. This will be supplemented with seminar courses on current topics in industrial and scientific areas, including fermentations involving recombinant organisms, bioproduct recovery (including macromolecular separations), site-directed mutagenesis techniques, metabolic regulation, enzyme inhibitor design and the application of enzymes and antibodies as catalysts in organic syntheses. Lectures from internationally known guests in a variety of related disciplines will further enrich the training program. Research will be conducted in the various area described above under the supervision of the faculty mentors. Trainees Predoctoral students will enter the program with varying backgrounds, all holding Baccalaureate degrees in engineering or science (some with Masters degrees). They will be selected on the basis of undergraduate scholastic performance, scores on GRE tests and recommendations from faculty at their undergraduate institutions. Support for 12 trainees is requested. The average duration of the doctoral program in the participating departments is 5.5 years.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Institutional National Research Service Award (T32)
Project #
2T32GM008352-11
Application #
2721440
Study Section
National Institute of General Medical Sciences Initial Review Group (BRT)
Project Start
1989-09-27
Project End
2004-06-30
Budget Start
1999-07-01
Budget End
2000-06-30
Support Year
11
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Engineering (All Types)
Type
Schools of Arts and Sciences
DUNS #
094878337
City
Berkeley
State
CA
Country
United States
Zip Code
94704

  Publications

Dietrich, Jeffrey A; Shis, David L; Alikhani, Azadeh et al. (2013) Transcription factor-based screens and synthetic selections for microbial small-molecule biosynthesis. ACS Synth Biol 2:47-58
Shen, Sam H; Wertz, Diana L; Klinman, Judith P (2012) Implication for functions of the ectopic adipocyte copper amine oxidase (AOC3) from purified enzyme and cell-based kinetic studies. PLoS One 7:e29270
Koerber, James T; Klimczak, Ryan; Jang, Jae-Hyung et al. (2009) Molecular evolution of adeno-associated virus for enhanced glial gene delivery. Mol Ther 17:2088-95
Stephanopoulos, Nicholas; Carrico, Zachary M; Francis, Matthew B (2009) Nanoscale integration of sensitizing chromophores and porphyrins with bacteriophage MS2. Angew Chem Int Ed Engl 48:9498-502
Marner 2nd, Wesley D; Shaikh, Afshan S; Muller, Susan J et al. (2009) Enzyme immobilization via silaffin-mediated autoencapsulation in a biosilica support. Biotechnol Prog 25:417-23
Kohen, Naomi T; Little, Lauren E; Healy, Kevin E (2009) Characterization of Matrigel interfaces during defined human embryonic stem cell culture. Biointerphases 4:69-79
Colaco, Martin; Park, Jun; Blanch, Harvey (2008) The kinetics of aggregation of poly-glutamic acid based polypeptides. Biophys Chem 136:74-86
Marner 2nd, Wesley D; Shaikh, Afshan S; Muller, Susan J et al. (2008) Morphology of artificial silica matrices formed via autosilification of a silaffin/protein polymer chimera. Biomacromolecules 9:1-5
Abranches, Elsa; O'Neill, Analeah; Robertson, Matthew J et al. (2006) Development of quantitative PCR methods to analyse neural progenitor cell culture state. Biotechnol Appl Biochem 44:1-8
Rothman, Steven C; Voorhies, Mark; Kirsch, Jack F (2004) Directed evolution relieves product inhibition and confers in vivo function to a rationally designed tyrosine aminotransferase. Protein Sci 13:763-72

Showing the most recent 10 out of 20 publications