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Microbial cultures growth conditions

Although exopolysaccharides do not normally have a structural role, they do form structures that can be detected by either light or electron microscopy. Exopolysaccharides may form part of a capsule closely attached to the microbial cell surface, or appear as loose slime secreted by the cell but not directly attached to it mucoid Exopolysaccharide producing cells usually form mucoid colonies on solid media and colonies liquid cultures of these cells may become very viscous. However, growth conditions can... [Pg.195]

A strain of Azotobacter vinelandii was cultured in a 15 m3 stirred fermenter for the production of alginate. Under current conditions the mass transfer coefficient, kLa, is 0.18 s. Oxygen solubility in the fermentation broth is approximately 8 X 10 3 kgm-3.9 The specific oxygen uptake rate is 12.5 mmol g 1 h. What is the maximum cell density in the broth If copper sulphate is accidentally added to the fermentation broth, which may reduce the oxygen uptake rate to 3 mmol g 1 h 1 and inhibit the microbial cell growth, what would be the maximum cell density in this condition ... [Pg.20]

P, mainly in the form of RNA and DNA, polyphosphates and phospholipids, with minor amounts of other P-containing cell biochemicals like adenosine phosphates. Measurement of the P content of the microbial biomass is an essential prerequisite for assessing its role in the P cycle, and its effect on plant nutrition. Until very recently, estimates of microbial P have had to be made from microbial biomass measurements, and literature values for the P contents of laboratory cultured microorganisms which can vary widely depending on growth conditions. ... [Pg.337]

It is necessary to estabUsh a criterion for microbial death when considering a sterilization process. With respect to the individual cell, the irreversible cessation of all vital functions such as growth, reproduction, and in the case of vimses, inabiUty to attach and infect, is a most suitable criterion. On a practical level, it is necessary to estabUsh test criteria that permit a conclusion without having to observe individual microbial cells. The failure to reproduce in a suitable medium after incubation at optimum conditions for some acceptable time period is traditionally accepted as satisfactory proof of microbial death and, consequentiy, stetihty. The appHcation of such a testing method is, for practical purposes, however, not considered possible. The cultured article caimot be retrieved for subsequent use and the size of many items totally precludes practical culturing techniques. In order to design acceptable test procedures, the kinetics and thermodynamics of the sterilization process must be understood. [Pg.404]


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Cultural conditions

Culture conditions

Growth conditions

Microbial conditions

Microbial cultures

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