Preparation of α1- and α2-isomers of mono-Ru-substituted Dawson-type phosphotungstates with an aqua ligand and comparison of their redox potentials, catalytic activities, and thermal stabilities with Keggin-type derivatives.

Both the α1- and the α2-isomers of mono-ruthenium (Ru)-substituted Dawson-type phosphotungstates with terminal aqua ligands, [α1-P2W17O61Ru(III)(H2O)](7-) (α1-RuH2O) and [α2-P2W17O61Ru(III)(H2O)](7-) (α2-RuH2O), were prepared in pure form by cleavage of the Ru-S bond of the corresponding DMSO derivatives, [α1-P2W17O61Ru(DMSO)](8-) (α1-RuDMSO) and [α2-P2W17O61Ru(DMSO)](8-) (α2-RuDMSO), respectively. Redox studies indicated that α1-RuH2O and α2-RuH2O show proton-coupled electron transfer (PCET), and the Ru(III)(H2O) species was reversibly reduced to Ru(II)(H2O) species and oxidized to Ru(IV)([double bond, length as m-dash]O) species and further to Ru(V)([double bond, length as m-dash]O) species in aqueous solution depending on the pH. Their redox potentials and thermal stabilities were compared with those of the corresponding α-Keggin-type derivatives ([α-XW11O39Ru(H2O)](n-); X = Si(4+) (n = 5), Ge(4+) (n = 5), or P(5+) (n = 4)). The basic electronic and redox features of Ru(L)-substituted Keggin- and Dawson-type heteropolytungstates (with L = H2O or O(2-)) were analyzed by means of density functional calculations. Similar to the corresponding α-Keggin-type derivatives, both α1-RuH2O and α2-RuH2O show catalytic activity for water oxidation.

Dextran sulfate-induced degradation of spontaneously apoptotic B cells.

Mature resting mouse splenic B cells undergo spontaneous apoptosis in vitro, unless rescued by specific agents including interleukin 4 and protein kinase C activators. Dextran sulfate, a B cell activator, has been reported to have such a protective effect on B cell apoptosis. This study was undertaken to elucidate the mechanism underlying the protective effect of dextran sulfate. The ratio of apoptotic B cells gradually increased to about one third with 24 h of incubation. Dextran sulfate dose-dependently reduced apoptotic cells, but it did not cause concomitant increase in viable cells. Both DNA levels and lactate dehydrogenase activities in the supernatants of dextran sulfate-treated cultures were significantly higher than those in the supernatants of untreated cultures. Concomitantly, DNA levels and lactate dehydrogenase activities in the cell pellets of dextran sulfate-treated cultures were lower than those in the cell pellets of untreated cultures. Addition of dextran sulfate to the culture of B cells 18 h after the start of incubation, when about one fifth of the B cells were dead, significantly reduced apoptotic cells during the next 6-h incubation. This decrease in the number of apoptotic cells was detectable as early as 1 h after addition of dextran sulfate and was prevented by Zn(2+), Co(2+), Ni(2+), the serine protease inhibitor 4-(2-aminoethyl)benzenesulfonyl fluoride (AEBSF) or incubation on ice. These results indicated that dextran sulfate treatment did not prevent apoptosis but rather promoted degradation of apoptotic cells and suggest the involvement of DNase and protease in this process.

Induction of cytolytic activity and interferon-gamma production in murine natural killer cells by polymyxins B and E.

Natural killer (NK) cells are the primary effector cells of the innate immune system and have well-established roles in tumor rejection and resistance to viruses, bacteria and certain parasites. There is a need for more specific immune modulators of NK cell activity that lack the wide-ranging side effects of NK cell-stimulatory interleukins. The polycationic antibiotic polymyxin B (PMB) has been shown to have a unique ability to enhance activities of some immune cells, independent of its antibiotic properties. Here we report that both PMB and its analog polymyxin E (PME) markedly enhanced the activity of NK cells enriched from the murine spleen. Maximal activation of NK cell activity was obtained after 24 h of incubation with PMB at a dose of 300 mug/ml. PMB nonapeptide, one of the two PMB domains, and PME methanesulfonate, the negatively charged derivative of PME, had little effect on NK cell activity. PMB induced interferon (IFN)-gamma and tumor necrosis factor-alpha production in NK cells. Proliferation of NK cells in vitro was significantly stimulated by being incubated with PMB. Administration of PMB to mice for 7 consecutive days stimulated splenic NK cell activity and increased NK cell populations in the spleen. These results suggest that the polycationic antibiotics PMB and PME may up-regulate innate and adaptive immune responses by induction of NK cell activity and IFN-gamma production.

Differentiation of murine B cells induced by chondroitin sulfate B.

A two-step culture system was used to investigate the role of chondroitin sulfate (CS) B, which is mitogenic to B cells, in differentiation of B cells. Mouse spleen B cells were incubated for 3 days with CSB in the presence of interleukin (IL)-4 and IL-5. After washing, the cells were replated at 10(5) viable cells/well and recultured without CSB in the presence of IL-4 and IL-5. CSB dose-dependently increased IgM production, the greatest enhancement being 450%. Dextran sulfate had a similar effect, whereas other glycosaminoglycans, CSA, CSC, heparin and hyaluronic acid, were marginally effective. Treatment of B cells with CSB resulted in increases in the number of IgM-secreting cells and numbers of CD138-positive cells and CD45R/B220-negative cells. CSB-induced IgM production was inhibited by the protein kinase C (PKC) inhibitor GF109203X but not by the phosphatidylinositol 3-kinase (PI3K) inhibitor wortmannin. These results demonstrated that CSB promoted differentiation of B cells in the presence of IL-4 and IL-5 and suggested that PKC but not PI3K is crucial for CSB-induced IgM production.