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To study the dynamics of free liquid films which are stabilized with ionic surfactants, an electrohydrodynamic theory is developed. The long-range interaction forces, namely the repulsive force arising from the overlap of diffuse electric double layers and the attractive Van der Waals-London force, are described by the Maxwell stress tensor with its related field equations and the Van der Waals potential. The short-range surface force has a normal Laplace component and a tangential surface tension gradient component. The total set of first-order equations and their boundary conditions, which describes the capillary waves on the surfaces and the induced flow motion in the film, has been solved. The dispersion relation for the “squeezing mode” is obtained. The cases of no-slip condition and the long-wavelength limit have been studied in more detail. The testability of the dispersion relation using laser beat spectroscopy is reported.  相似文献   
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Introduction 2, 3-Dichloro-5, 6-dicyanobenzoquinone (DDQ) can react with lignans of the mono- arylidene-butyrolactone1, aryltetralin2, dibenzylbutane3 and aryltetralin-butyrolactone4,5 series. We have studied the reactions of this reagent with podophyllotoxin 1, which is a well-known natural product on account of its long history of use in folk medicine and the biological activity of its many derivatives6. In particular, derivatives of 4-demethyl epipodophyllotoxin are used in cancer chemo…  相似文献   
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BACKGROUND: The identification of cellular targets has traditionally been the starting point for natural product mode of action studies and has led to the understanding of many biological processes. Conventional experimental approaches have depended on cell-based screening and/or affinity chromatography. Although both of these techniques aid in the discovery of protein cellular targets, a method that couples protein identification with gene isolation would be extremely valuable. RESULTS: A procedure for the direct cloning of cellular proteins, based on their affinity for natural products, using cDNA phage display has been developed. The technique is referred to as display cloning because it involves the cloning of proteins displayed on the surface of a bacteriophage particle. The approach has been established by isolating a full-length gene clone of FKBP12 (FK506-binding protein) from a human brain cDNA library using a biotinylated FK506 probe molecule. During the affinity selection, the FKBP12 gene emerged as the dominant library member and was the only sequence identified after the second round of selection. CONCLUSIONS: The development of display cloning greatly facilitates the investigation of ligand-receptor interaction biology and natural product mode of action studies. This procedure utilizes heterologous protein display on infectious phage, which allows the amplification and repeated selection of putative sequences, leading to unambiguous target identification. In addition, the direct connection of a functional protein to its gene sequence eliminates the subsequent cloning step required with tissue homogenate or cell lysate affinity methods, allowing direct isolation of an expressible gene sequence.  相似文献   
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