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In Vitro Experiments

It is also clear that it is difficult to relate cause and effect to any specific chemical since, with the exception of point source effluents, many waterways contain a multitude of chemicals, of which the active endocrine disruptor may not be that which has been measured in the water or tissue. For such reasons, many studies have used in vitro experiments in which isolated tissue, either from a control animal or one captured in a polluted water system, is exposed to a single pollutant in the laboratory. Such experiments have shown significant disruption to testicular activity by a wide range of xenobiotics, including cadmium, lindane, DDT, cythion, hexadrin and PCBs. ... [Pg.36]

Consequently, biochemists conducting in vitro experiments were limited in their choice of buffers effective at or near physiological pH. In 1966, N.E. Good devised a set of synthetic buffers to remedy this problem, and over the years the list has expanded so that a good selection is available (Figure 2.18). [Pg.52]

In in vitro experiments, caldesmon can inhibit the activation of myosin by actin and this inhibition can be reversed by calmodulin. Thus, there is a potentiality for... [Pg.176]

Why are the oceans so depleted in these trace metals Certainly it is not for the lack of availability from rock weathering or because of constraints imposed by the solubility of any unique compound of these elements. The reason must lie in the dynamics of the system of delivery of the metals to the oceans and their subsequent behavior in an ocean that cannot be simulated by simple in vitro experiments involving homogeneous reaction kinetics. [Pg.402]

Consequently, the antioxidant activity of GA in biological systems is still an unresolved issue, and therefore it requires a more direct knowledge of the antioxidant capacity of GA that can be obtained by in vitro experiments against different types of oxidant species. The total antioxidant activity of a compound or substance is associated with several processes that include the scavenging of free radical species (eg. HO, ROO ), ability to quench reactive excited states (triplet excited states and/ or oxygen singlet molecular 1O2), and/or sequester of metal ions (Fe2+, Cu2+) to avoid the formation of HO by Fenton type reactions. In the following sections, we will discuss the in vitro antioxidant capacity of GA for some of these processes. [Pg.11]

One major finding of this study was that the polymeric implants remained intact throughout the 1-year course of the experiments, in complete agreement with the predictions based on in vitro experiments. [Pg.209]

Discovery of Kanamycin, and Establishment oflMC. Chloramphenicol, chlor- and oxy-tetracyclines, and pyridomycin (H. Umezawa, 1967) were active, in in vitro experiments, against strains of tuberculosis, but these drugs, in contrast to streptomycin, were clinically inactive. H. Umezawa... [Pg.6]

The formation of the PIC described above is based on the sequential addition of purified components in in vitro experiments. An essential feature of this model is that the assembly takes place on the DNA template. Accordingly, transcription activators, which have autonomous DNA binding and activation domains (see Chapter 39), are thought to function by stimulating either PIC formation or PIC function. The TAF coactivators are viewed as bridging factors that communicate between the upstream activators, the proteins associated with pol II, or the many other components of TFIID. This view, which assumes that there is stepwise assembly of the PIC—promoted by various interactions between activators, coactivators, and PIC components— is illustrated in panel A of Figure 37-10. This model was supported by observations that many of these proteins could indeed bind to one another in vitro. [Pg.351]

Nonvolatile Nitrosamines In Saliva. In vitro experiments had indicated that the tobacco-specific nitrosamines are formed also during snuff dipping (26). Therefore, we analyzed the saliva of snuff dippers and tobacco chewers. A comparison of the results demonstrated the presence of TSNA in saliva at a wide range of concentrations (Table Vl), which could be ascribed to differences in the product, but also to differences in the manner of chewing, and, lastly, to individual factors in each person s saliva. [Pg.262]

Preliminary studies, which have repeated many of the in vitro experiments in vivo, reported that the differentiation between stratum corneum and viable epidermis is at least as good, if not better in vivo and that many of the other experiments are similarly reproduced [16]. [Pg.103]

A semi-interpenetrated network was obtained by bulk polymerization of 2-hydroxye-thyl methacrylate incorporated in DMF treated PET films by solvent-exchange technique, followed by treatment of films in e-lectrical discharges. Heparinization was accomplished by reacting glutaraldehyde with heparin and poly(2-hydroxyethyl methacrylate) present on the surface of modified polyester films. The immobilization of heparin was indirectly evidenced by chromatographying the silylated hydrolyza-tes of heparinized PET films and heparin, respectively. In vitro experiments demonstrated the enhanced thromboresistance of heparinized films. [Pg.229]

For over three decades, laboratory research has shown caffeine to be effective at mobilizing calcium in skeletal muscle. In vitro experiments have amply demonstrated that caffeine lowers the excitability threshold and extends the length of muscular contractions via calcium release from the sarcoplasmic reticulum.1012 Caffeine also inhibits calcium reuptake by the sarcoplasmic reticulum, perpetuating calcium availability for muscle work.1318 Also, caffeine promotes increased twitch tension development in muscles.1718... [Pg.240]

These diffusivities are estimates obtained by in vitro experiment (stratum corneum) or by comparison with small tissues in which diffusivities have been measured (all others). They do not account for regional variations across the body surface, so on both counts must be considered highly approximate. [Pg.214]

There have been attempts to conduct in vitro experiments in a manner that gives more meaningful data with regard to lung deposition. These methods, which are loosely based on inertial impaction, utilize inspiratory flow cycles rather than fixed flow... [Pg.497]

Combined use of Eqs. (43)—(45) allows free drug concentrations to be predicted for each subcompartment. This approach to modeling free drug concentrations would make use of protein binding parameters (i.e., Bt, Kt) obtained from in vitro experiments. [Pg.87]

Protein binding parameters B, and Kh as depicted in Eq. (44), are obtained from in vitro experiments utilizing filtration, centrifugation, and dynamic dialysis or equilibrium dialysis methods. These techniques have been reviewed elsewhere [54,55],... [Pg.96]

Note For the in vitro experiments the corresponding cell staining was 5.3% and 52.9%. [Pg.293]


See other pages where In Vitro Experiments is mentioned: [Pg.191]    [Pg.494]    [Pg.47]    [Pg.128]    [Pg.1083]    [Pg.174]    [Pg.433]    [Pg.445]    [Pg.192]    [Pg.310]    [Pg.204]    [Pg.227]    [Pg.142]    [Pg.175]    [Pg.164]    [Pg.9]    [Pg.541]    [Pg.309]    [Pg.310]    [Pg.169]    [Pg.205]    [Pg.666]    [Pg.286]    [Pg.112]    [Pg.304]    [Pg.33]    [Pg.131]    [Pg.218]    [Pg.34]    [Pg.118]    [Pg.51]    [Pg.6]    [Pg.94]    [Pg.542]   
See also in sourсe #XX -- [ Pg.355 ]

See also in sourсe #XX -- [ Pg.420 ]




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Boyds in vitro experiment and other related experiments

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