Your search keyword '"Hampel WA"' showing total 3 results

1. High cell density cultivation of Brevibacterium linens and formation of proteinases and lipase.

Author

Adamitsch BF, Karner F, and Hampel WA

Subjects

Ammonium Sulfate pharmacology, Brevibacterium classification, Brevibacterium drug effects, Cell Count, Cells, Cultured, Culture Media pharmacology, Endopeptidases biosynthesis, Enzyme Activation, Lactic Acid pharmacology, Leucyl Aminopeptidase biosynthesis, Peptones pharmacology, Quality Control, Soybean Proteins pharmacology, Species Specificity, Brevibacterium enzymology, Brevibacterium growth & development, Cell Culture Techniques methods, Lipase biosynthesis

Abstract

Brevibacterium linens forms hydrolytic enzymes which can be used to accelerate the ripening of cheese without causing bitterness. B. linens ATCC 9172 was grown to a high cell density (50 g dry wt l-1 after 60 h) in a mineral medium containing lactic acid, soy-peptone and ammonium sulphate by applying a continuous feed of nutrients. The maximal activities of L-leucine aminopeptidase and cell-associated proteinase were 286 U l-1 and 202 U l-1, respectively. The cell-associated lipolytic activity exhibited a strong and sudden increase at 46 h, resulting in a maximum of 9.5 U g-1 dry wt; thus the volumetric productivity of proteolytic and lipolytic activity was 4220 U l-1 h-1 and 7.3 U l-1 h-1, respectively.

Published

2003

2. A synthetic medium for continuous culture of the S-layer carrying Bacillus stearothermophilus PV 72 and studies on the influence of growth conditions on cell wall properties.

Author

Schuster KC, Mayer HF, Kieweg R, Hampel WA, and Sára M

Abstract

Bacterial cell surface layers (S-layers) which show a crystalline structure, defined pores, and a regular arrangement of functional groups can be used for production of isoporous ultrafiltration membranes and as a matrix for immobilization of macromolecules. S-layer-carrying cell wall fragments from thermophilic Bacillaceae possess an extremely thin peptidoglycan-containing layer with pores larger than those in the S-layer lattice. Thus, they can directly be used for biotechnological applications, when an S-layer protein pool is stored in the rigid cell wall layer which is released during cell wall preparation, forming an inner S-layer. In the present study, a synthetic medium for Bacillus stearothermophilus PV 72 was developed by applying the pulse and shift technique with the aim to produce cell wall fragments with before-mentioned properties by varying the growth conditions in continuous culture. The organism was grown at 57 degrees C in a bioreactor with 1 L working volume equipped with exhaust gas analysis and connected to a PC-based process control system. Biomass concentration was 2.2 g/L out of 8 g/L glucose at a dilution rate of 0.3 h(-1), giving a biomass productivity of 0.66 g/L h. Although the organism was grown under different conditions, no change in peptidoglycan composition, extent of peptidoglycan crosslinking, and content of secondary cell wall polymers was observed. The amount of S-layer protein pool stored in the rigid cell wall layer and the autolytic activity depended mainly on the specific growth rate. Cell wall fragments with properties required for ultrafiltration membrane production could be produced by parameter settings in continuous culture.

Published

1995

3. Differential effects of general amino acid control of lysine biosynthesis on penicillin formation in strains of Penicillium chrysogenum.

Author

Hönlinger C, Hampel WA, Röhr M, and Kubicek CP

Subjects

2-Aminoadipic Acid analysis, 2-Aminoadipic Acid biosynthesis, Aldehyde Oxidoreductases pharmacology, Amino Acids analysis, Amitrole pharmacology, Chromatography, High Pressure Liquid, L-Aminoadipate-Semialdehyde Dehydrogenase, Penicillium chrysogenum enzymology, Amino Acids pharmacology, Lysine biosynthesis, Penicillins biosynthesis, Penicillium drug effects, Penicillium chrysogenum drug effects

Published

1988