Characterization of three monoclonal antibodies which induce and modulate superoxide anion generation in guinea pig macrophages

Three monoclonal antibodies (Ab), termed KY 12, KY 22, and KY 25 and raised against guinea pig macrophages, induced superoxide anion (O2-) generation in the cells. Although each monoclonal Ab bound to macrophages, each had a different pattern of binding to other cell types. In response to each of the Ab, the amount of O2- generated by 5 X 10(5) macrophages was between 0.5 and 0.7 nmol/min and was augmented threefold to fivefold by the addition of F(ab')2 fragments of rabbit Abs to mouse Ig. When macrophages were pretreated with soluble immune complexes (I.C.) prior to stimulation by the monoclonal Ab, the O2- generation stimulated by KY 12 or KY 22 was reduced by more than 70%. In contrast, pretreatment of macrophages with I.C. did not reduce O2- generation in response to KY 25. KY 12 and KY 22 stimulated adenyl cyclase activity in macrophages, but KY 25 did not. Pretreatment of the cells with soluble I.C. did not interfere with the enhancing effect of the monoclonal Ab on adenyl cyclase activity. Pretreatment of macrophages with KY 12 reduced by over 60% of subsequent generation of O2- in response to wheat germ agglutinin, I.C., formyl-methionyl-leucyl-phenylalanine, phorbol myristate acetate, KY 22, or KY 25. KY 22 or KY 25 did not suppress the generation of O2- in response to other stimuli. These results suggest that KY 22 and KY 25 activate O2- generation in a manner that differs from that of KY 12. These monoclonal Ab should prove useful in examining the regulation of O2- production.     

The cyclic GMP-induced inward current in neuron R14 of Aplysia californica: similarity to a FMRFamide-induced inward current

Injecting cGMP into Aplysia neuron R14 induced an inward current similar to one elicited by application of FMRFamide to the outside of that cell. In contrast, injection of cAMP into R14 caused a long-lasting outward current and conductance increase. Phosphodiesterase inhibitors increased the cGMP and FMRFamide-induced inward currents in R14. The cGMP-induced inward current is voltage dependent and is largely carried by Na+. It is also strongly and inversely dependent on both external [Ca2+] and [Cl-], although these ions are not significant current carriers. Changing external [K+] had no effect. Voltage and ion dependencies of the cGMP-induced inward current are similar to those of an inward current induced by FMRFamide. Thus cGMP may be a second messenger to FMRFamide in producing a slow inward current in R14. cGMP does not appear to be a second messenger to FMRFamide in most Aplysia neurons.     

Nonisometric behavior of fascicles during isometric contractions of a human muscle

Fascicle length, pennation angle, and tendonelongation of the human tibialis anterior were measured in vivo byultrasonography. Subjects (n = 9) wererequested to develop isometric dorsiflexion torque gradually up tomaximal at the ankle joint angle of 20° plantarflexion from theanatomic position. Fascicle length shortened from 90 ± 7 to 76 ± 7 (SE) mm, pennation angle increased from 10 ± 1 to 12 ± 1°, and tendon elongation increased up to 15 ± 2 mm with gradedforce development up to maximum. The tendon stiffness increased withincreasing tendon force from 10 N/mm at 0-20 N to 32 N/mm at240-260 N. Young's modulus increased from 157 MPa at 0-20 Nto 530 MPa at 240-260 N. It can be concluded that, in isometriccontractions of a human muscle, mechanical work, some of which isabsorbed by the tendinous tissue, is generated by the shortening ofmuscle fibers and that ultrasonography can be used to determine thestiffness and Young's modulus for human tendons.

     

Short-day flowering of Lemna gibba G3 induced by salicylic acid

Salicylic acid, probably as a chelating agent of the EDTA-salicylaldoximetype, can eliminate the light requirement during the inductivephase of Lemna gibba G3, and thus is able to induce short-dayflowering of this long-day plant. (Received September 4, 1975; )     

Induction of two K+ currents by complement component C5a in mouse macrophages.

Puff application of complement component C5a (5 x 10(-8) M) onto peritoneal macrophages from thioglycollate-stimulated mice induced two kinds of outward current at a holding potential of -68 mV, a slowly-rising sustained outward current and a spike-like transient outward current. Quinidine (2 x 10(-4) M) and tetraethylammonium (10(-2) M) partially suppressed both types of outward current. Charybdotoxin (2 x 10(-6) M) markedly suppressed the spike-like outward current. Reversal potentials in bath solutions of different external K+ concentrations were dependent only on K+ concentrations. The transient current was not suppressed in Ca(2+)-free EGTA-containing solution, but was completely abolished in BAPTA-containing solution. One kind of single channel responding to C5a, which has a single-channel conductance of 29 pS, was recorded from cell-attached patches. These results suggest that C5a activates a Ca(2+)-dependent and another type of K+ current.     

Regulation of Polyphosphoinositide Metabolism in Pea Plasma Membranes by Elicitor and Suppressor from a Pea Pathogen, Mycosphaerella pinodes

Effects of the elicitor and the suppressor from a pea pathogen,Mycosphaerella pinodes, on polyphosphoinositide metabolism inpea plasma membranes were examined in vitro. Lipid phosphorylationin the isolated pea plasma membrane was drastically stimulatedby the elicitor, but markedly inhibited by the suppressor. Asimilar inhibitory effect was observed by the treatment withorthovanadate or K-252a that blocked pisatin production inducedby the elicitor. Neomycin, an aminoglycoside antibiotic thatinteracts with the polyphosphoinositide metabolism, also affectedthe lipid phosphorylation in vitro and blocked the elicitor-inducedaccumulation of pisatin in vivo. These results suggest thatrapid changes of polyphosphoinositide metabolism in pea plasmamembranes is one of indispensable processes during the elicitationof defense responses. (Received January 22, 1992; Accepted March 23, 1992)     

Enzymatic properties of cytochrome P450 catalyzing 3′-hydroxylation of naringenin from the white-rot fungus Phanerochaete chrysosporium

We cloned full-length cDNAs of more than 130 cytochrome P450s (P450s) derived from Phanerochaete chrysosporium, and successfully expressed 70 isoforms using a co-expression system of P. chrysosporium P450 and yeast NADPH-P450 reductase in Saccharomyces cerevisiae. Of these P450s, a microsomal P450 designated as PcCYP65a2 consists of 626 amino acid residues with a molecular mass of 68.3 kDa. Sequence alignment of PcCYP65a2 and human CYP1A2 revealed a unique structure of PcCYP65a2. Functional analysis of PcCYP65a2 using the recombinant S. cerevisiae cells demonstrated that this P450 catalyzes 3′-hydroxylation of naringenin to yield eriodictyol, which has various biological and pharmacological properties. In addition, the recombinant S. cerevisiae cells expressing PcCYP65a2 metabolized such polyaromatic compounds as dibenzo-p-dioxin (DD), 2-monochloroDD, biphenyl, and naphthalene. These results suggest that PcCYP65a2 is practically useful for both bioconversion and bioremediation.