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Transfection structures

Urotensin II Receptor (GPR14). The vasoactive cyclic peptide urotensin II (U-II) is the endogenous ligand of the G protein-coupled orphan receptor GPR14. Structure-activity relationships from 25 peptide analogs, which mobilize intracellular calcium in GPR14-transfected CHO cells, and the... [Pg.387]

Activated PAMAM dendrimers interact with DNA to form a DNA-dendrimer complex with a toroid-like structure (Fig. 2). Such DNA-dendrimer complexes have diameters of 50-100 nm [10],which means that the DNA molecules are highly condensed in these complexes. A 6-kb plasmid alone, for example, has an extended structure several hundred nanometers in diameter. In transfection experiments, typically an 8- to 12-fold excess of positive amino groups over negatively... [Pg.232]

When assayed in HEK293 cells transfected with the cloned human, rat and guinea pig TRPVl, (23a) showed similar potencies. Not unexpeetedly, (23a) showed poor metabolic stability and a structure-activity study to optimize potency and drug-like properties was initiated. Modification on the left-handed A -aryl section showed that ... [Pg.161]

Geisse, S. and Henke, M. (2005) Large-scale transient transfection of mammalian cells a newly emerging attractive option for recombinant protein production. Journal of Structural and Functional Genomics, 6 (2-3), 165-170. [Pg.58]

The advantage of mRNA over plasmid transfection is the ability of in vitro transcription to allow precise control over features contained within the mRNA (Humphreys et al., 2005 Pillai et al., 2005 Westman et al, 2005). For example, mRNA can be prepared either with or without the physiological m7G(5/)ppp(5/)G cap structure and S poly(A) tail, which are important mediators of canonical translation initiation (Gallie, 1991 Hentze et al., 2006 Iizuka et al, 1994 Kahvejian et al, 2005 Tarun and Sachs, 1995). [Pg.122]

In our work, we opted to deploy the IRES sequences within the 5 UTR of mono-cistronic reporter mRNA (Humphreys el al, 2005 Fig. 6.IB), which were directly transfected into HeLa cells. IRES-containing transcripts were further capped with the nonphysiological A(5/)ppp(5/)G cap structure,... [Pg.126]

In Fig. 9.4, the results are shown of an experiment using a double (annexinA4-EYFP+ annexinA4-mCherry) transfected cell immediately after addition of the calcium ionophore ionomycin (top) and 5 min after application of ionomycin (bottom). Clearly visible is the diffuse localization of annexin A4 before relocation and the more structured localization (into membrane ruffles and filopodia) after relocation. More importantly, the EYFP fluorescence lifetime is quenched from 2.9 ns before translocation to... [Pg.417]

The principal difference in the overall protein composition of PNS and CNS myelin is that P0 replaces PLP as the major protein, although myelin-forming Schwann cells do express very low levels of PLP. It is interesting to note that PLP and P0 proteins, which are so different in sequence, post-translational modifications and membrane topology, may have similar roles in the formation of structures as closely related as myelin of the CNS and PNS respectively. Expression of P0 in transfected cells results in cell-cell interactions that are due to homophilic binding... [Pg.63]

The curvature effect of the double helix of DNA, caused by the binding of dimers of active receptors to the HRE sequences, has been obtained by means of experiments of transfection of lineal DNA structures to cells that previously did not express the gene under study. The reality of the cells in vivo must be... [Pg.44]

Because the fMet-Leu-Phe receptor is present only at low levels in neutrophils (-12 x 10 15 g of receptor per cell), it has proved difficult to purify and characterise. Researchers have therefore turned to molecular cloning techniques to gain insight into the molecular structure of this receptor. This approach itself has not been easy because, in the absence of an antibody that specifically binds to the receptor, or else without some amino acid sequence data that can be used to synthesise oligonucleotide probes, cDNA libraries cannot be screened to isolate relevant clones. Therefore, experimental systems in which functional fMet-Leu-Phe receptors are expressed on the surfaces of transfected cells have been used. Two main systems have been utilised expression of mRNA injected into Xenopus laevis oocytes and cDNA cloning into the COS-cell expression vector. [Pg.98]

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