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Blood 89, 1896-1904. Human platelets display high-affinity receptors for thrombopoietin. 1997

Broudy, V.C., Lin, N.L., Sabath, D.F., Papayannopoulou, T. and Kaushansky, K.

Notes: In this study, Poly(A)+ RNA was isolated from B16 melanoma cell total RNA using the PolyATtract® mRNA Isolation System. The isolated RNA was used for cDNA library construction. The RNAgents® Total RNA Isolation System was used to isolate total RNA from HEL and K562 human erythroleukemia cells. The isolated RNA was used for RT-PCR. RNasin® Ribonuclease Inhibitor was used in a very innovative fashion. Peripheral mononuclear cells isolated from blood were directly lysed in a hypotonic buffer containing the inhibitor. The lysates from these cells were used directly for RT-PCR. (2026)

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Cell 88(3), 385-392. Mutation of the Ca2+ channel b subunit gene Cchb4 is associated with ataxia and seizures in the lethargic (lh) mouse. 1997

Burgess, D.L., Jones, J.M., Meisler, M.H. and Noebels, J.L.

Notes: Poly(A)+ RNA was isolated from mouse brain total RNA and used for Northern analysis. The authors used Promega's PolyATtract® mRNA Isolation System, AMV Reverse Transcriptase and RNasin® Ribonuclease Inhibitor in this study. (2104)

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Cell 88, 385-392. Mutation of the Ca2+ Channel beta Subunit Gene Cchb4 Is Associated with Ataxia and Seizures in the Lethargic (lh) Mouse. 1997

Burgess, D., Jones, J., Meisler, M., Noebels, J.

Notes: AMV Reverse Transcriptase, PolyATtract® mRNA Isolation System, dNTPs, RNasin® Ribonuclease Inhibitor. (1930)

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J. Neurosci. 17, 6974-6987. Selective expression of insulin-like growth factor II in the songbird brain. 1997

Holzenberger, M., Jarvis, E.D., Chong, C., Grossman, M., Nottebohm, F. and Scharff, C.

Notes: T7 RNA Polymerase and SP6 RNA Polymerase were used to produce RNA probes labeled with digoxygenin-11-UTP. Transcripts were made in the presence of RNasin® Ribonuclease Inhibitor in a standard transcription reaction. The ribonucleotides ATP, CTP and GTP were used at 1mM. Both UTP and digoxygenin-11-UTP were used at 0.5mM in the reaction. The RNA probe was used for in situ hybridization. (1563)

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J. Exp. Med. 185, 695-706. The Immunodominant Antigen of an Ultraviolet-induced Regressor Tumor Is Generated by a Somatic Point Mutation in the DEAD Box Helicase p68. 1997

Dubey, P., Hendrickson, R., Meredith, S., Siegel, C., Shabanowitz, J., Skipper, J., Engelhard, V., Hunt, D., Schreiber, H.

Notes: Promega's Taq DNA Polymerase, RNasin® Ribonuclease Inhibitor, and fmol® DNA cycle Sequencing System were used in this study. (1952)

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Nucl. Acids Res. 24(5), 970-976. A binding factor for interleukin 2 mRNA. 1996

Hua, J. and Paetkau, V.

Notes: Jurkat cells, a human T lymphocyte line that can be induced to synthesize and secrete interleukin 2, contain a factor that binds interleukin 2 mRNA. The binding is sequence specific and occurs in the 3’-non-coding region, within 160nt of the end of the coding region, at or near a site on the mRNA that is rich in A and U residues. However, it appears not to be due to known AU binding factors. The factor is protease sensitive and binds non-covalently to interleukin 2 mRNA. It behaves like aprotein of molecular weight 50,000-60,000 after UV-induced cross-linking to the mRNA. Preparations of the binding factor also protect interleukin 2 mRNA against degradation by a recently described RNasin-resistant endoribonuclease activity in Jurkat cells. Protection occurs under the same conditions required to generate the gel-retarded complex. (1645)

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J. Clin. Invest. 97(7), 1761-1766. CD40 expression by human peripheral blood eosinophils. 1996

Ohkawara, Y., Xing, K., Glibetic, M., Nakano, K., Dolovich, J., Croitorus, K., Weller, P. and Jordana, M.

Notes: These authors used Promega's AMV Reverse Transcriptase, RNasin® Ribonuclease Inhibitor and Taq DNA Polymerase in this study. (2061)

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Immunity 5, 253-262. Cytotoxic T Cell-Resistant Variants Are Selected in a Virus-Induced Demyelinating Disease. 1996

Pewe, L., Wu, G., Barnett, E., Castro, R., Perlman, S.

Notes: Promega's Taq DNA Polymerase, fmol® DNA Cycle Sequencing System and RNasin® Ribonuclease Inhibitor were used in this study. (1954)

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Proc. Natl. Acad. Sci. USA 93, 15180-15184. Estrogen-induced transcription of the progesterone receptor gene does not parallel estrogen receptor occupancy. 1996

Lee, Y. and Gorski, J.

Notes: Promega's Taq DNA Polymerase, RNasin® Ribonuclease Inhibitor and M-MLV Reverse Transcriptase were used in this study. (2003)

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J. Clin. Invest. 98(8), 1851-1859. Prevention of adoptively transferred diabetes in nonobese diabetic mice with IL-10-transduced islet-specific Th1 lymphocytes: A gene therapy model for autoimmune diabetes. 1996

Moritani, M., Yoshimoto, K., Ii, S., Kondo, M., Iwahana, H., Yamaoka, T., Sano, T., Nakano, N., Kikutani, H. and Itakura, M.

Notes: Promega's RQ1 RNase-Free DNase, M-MLV Reverse Transcriptase and RNasin® Ribonuclease Inhibitor were used in this study. (2020)

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FEBS Lett. 343(1), 11-14. Modulation of cytosolic RNase activity by endogenous RNase inhibitor in rat vaginal epithelial cells on estradiol administration. 1994

Rao, K.S., Sirdeshmukh, R. and Gupta, P.D.

Notes: The cytosolic, alkaline RNase in rat vaginal epithelial cells (VEC) from normal, immature rats was found to be present largely in free, active form unlike in many other mammalian tissues where it is known to be present in a latent form as a complex with RNase inhibitor (RNasin). Estradiol (E2) administration induced expression of RNasin activity in the VEC from such animals and caused virtually total inhibition of cytosolic RNase activity in these cells by 12 h after hormone injection. These changes may have metabolic implications in relation to other biochemical events stimulated by estradiol in rat VEC. (1647)

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PCR Methods Appl. 3(6), 317-319. Rapid RT-PCR amplification from limited cell numbers. 1994

Edmands, S., Kirk, J., Lee, A., and Radich, J.

Notes: The inhibitor was used for protection of cells and colonies following RT-PCR. (1672)

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FEBS Lett. 328(3), 250-252. Endotoxin induces rat lung ribonuclease activity. 1993

Clerch, L.B., Wright, A. and Massaro, D.

Notes: Lipopolysaccharide (endotoxin), a component of gram-negative bacteria, causes marked alterations in eukaryotic gene expression and cellular physiology. We show that within one hour of injection of endotoxin into adult rats, there is an induction of ribonuclease activity in the lung. The degradation of RNA was prevented by treatment of the lung extract from endotoxin-injected rats with ribonuclease inhibitor (RNasin). We suggest that induction by endotoxin of ribonuclease activity is a novel mechanism by which cells could alter gene expression to meet an environmental challenge and caution that the presence of ribonuclease can hinder molecular biological analyses of tissue extracts from endotoxin-treated rats. (1644)

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J. Biol. Chem. 267, 21982-21986. Angiogenin is a cytotoxic, tRNA-specific ribonuclease in the RNase A superfamily. 1992

Saxena, S.K., Rybak, S.M., Davey, R.T., Jr, Youle, R.J., and Ackerman, E.J.

Notes: Protein synthesis was restored to angiogenin-injected oocytes by injecting RNasin® Ribonuclease Inhibitor plus total Xenopus or calf liver tRNAs. (1635)

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Genes Dev. 6, 1740–51.

Concentration-dependent activities of the even-skipped protein in Drosophila embryos.

1992

Manoukian, A.S., Krause, H.M,

Notes: RNasin Ribonuclease Inhibitor was used in the mRNA and protein localization steps. (4183)

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J. Biol. Chem. 266(31), 21208-21214. Comparison of RNases and toxins upon injection into Xenopus oocytes. 1991

Saxena, S.K., Rybak, S.M., Winkler, G., Meade, H.M., McGray, P., Youle, R.J. and Ackerman, E.J.

Notes: Recombinant angiogenin injected into oocytes abolished protein synthesis, and this toxic effect was inhibited by RNasin® Ribonuclease Inhibitor. (2248)

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