Tryptophan hydroxylation in cockroach (Periplaneta americana) nervous tissue was measured and compared to the hydroxylation of tryptophan in rat brain. Tryptophan hydroxylation in both tissues requires a pterine cofactor, and is inhibited by p-chlorophenylalanine. The molecular weight of the protein responsible for hydroxylation of tryptophan in cockroach nervous tissue obtained from gel filtration was estimated to be 54,000.The pH optima and enzyme kinetics differed greatly between the two hydroxylases. Hydroxylation of tryptophan by the enzyme obtained from cockroach tissues incubated with dimethyltetrahydropterine had a pH optimum of about 5.8–5.9 and a Km in crude enzyme preparations of 2.6 × 10−6 M and is activity was substrate inhibited above 10−4 M tryptophan. Hydroxylation of tryptophan by the enzyme obtained from rat brain incubated with dimethyltetrahydropterine had a pH optimum of about 6.5–7.0, a Km of about 6.7 × 10−4 M and exhibited no substrate inhibition at tryptophan concentrations up to 2 × 10−3 M.When incubated with biopterin, the presumed natural cofactor, the hydroxylase from cockroach tissues had a Km of about 6.8 × 10−5 M and no substrate inhibition occurred at tryptophan concentrations up to 2 × 10−3 M. Under the same conditions rat hydroxylase had a Km of 1.1 × 10−5M and substrate inhibition occurred above 10−4 M tryptophan.Unlike the mammalian situation, administration of tryptophan peripherally did not change the 5-hydroxytryptamine concentration in cockroach nervous tissue, but did increase tryptophan levels. The low Vmax values of the cockroach hydroxylase and the inability of administered tryptophan to elevate 5-hydroxytryptamine levels suggest that in the cockroach hydroxylation of tryptophan itself may be the limiting factor in the biosynthesis of 5-hydroxytryptamine. 相似文献
This report describes the measurement of estrogen and progesterone receptors in cytosols and nuclear fractions from endocervical tissue components. Unoccupied cytosol estrogen receptor levels as determined by Scatchard analysis of [3H]-estradiol binding data indicated a single class of high affinity binding sites for the epithelial-stromal complex (KD = 0.74 × 10−9 M). Binding was specific for estrogen (estradiol > estriol > estrone) and unaffected by desoxycorticosterone, dihydrotesterone and progesterone. Assays for total estrogen receptor verified that 71.6 ± 5.3% of this 8S estrogen receptor is in the epithelial-stromal complex while the remaining approximately 28% is localized in the stroma and fibromuscular wall, with the cells of the complex containing the highest receptor concentration. In 5-day pseudopregnant and ovariectomized rabbits compared to estrous rabbits there was a 50% decrease in the cytosol estrogen receptor in the epithelial-stromal complex and a 30% decrease in the concentration of nuclear receptor. Cytosol and nuclear progesterone receptors were measured as an indicator of estrogen action in the rabbit endocervix. Cytosol progesterone receptor concentrations (fmol/mg DNA) in 5-day pseudopregnant and ovariectomized animals were reduced to approximately 35% of the concentration in estrous animals. Nuclear progesterone receptor concentrations decreased 65% in 5-day pseudopregnant and 90% in ovariectomized animals suggesting decreased receptor synthesis. Collectively these data support the concept that the rabbit endocervix may be directly regulated by estrogens. 相似文献
Endothelin (ET) receptors on chondrocytes were demonstrated using cultured rabbit costal chondrocytes. After crosslinking the receptors on the cells with 125 I-ET-1, two major bands of 43 kDa and 46 kDa were separated by SDS-PAGE. Scatchard analysis demonstrated two classes of ET receptors with Kd values of 1 × 10?10 M and 5 × 10?9 M. The numbers of high- and low- affinity receptors were 1 × 104 and 2 × 105 per cell, respectively. The binding of ET-1 to chondrocytes was increased by treatment with PTH, DBcAMP, TGF-β1, IL-1β, RA and EGF. ET-1 stimulated DNA synthesis in cultured rabbit chondrocytes. ET-1 also stimulated calcium incorporation through the cell membrane of chondrocytes. These findings indicate that ET-1 has a physiological effect on chondrocytes via its receptors on the cells. 相似文献
Cytosol from the adrenal gland of male and female rats contains a specific binding protein for oestradiol-17β. This protein has all the characteristics of a cytoplasmic oestrogen receptor. It is excluded by Sephadex G-200 gel filtration, has a sedimentation coefficient of 8–9 S by sucrose density gradient centrifugation in low salt and dissociates into a 4 S form by centrifugation in high salt (0.5 M KCl). The binding protein is heat sensitive and oestradiol-17β binding is eliminated by protease and by sulphydryl blocking reagents (2mM p-chloromercuriphenylsulphonate). The bound oestradiol dissociates very slowly at 0°C. The adrenal oestrogen receptors have a very high affinity for oestradiol-17β, but lower affinity for oestradiol-17α and do not bind testosterone, androstene-3,17-dione or corticosterone. Scatchard analysis of the saturation data for oestradiol revealed one class of high affinity binding sites with an apparent equilibrium constant of dissociation KD at 0°C of 5.8 × 10−10M. The number of binding sites was calculated to be 70 fmol/mg cytosol protein. Cytosol fractions from androgen insensitive (tfm) male rats contain oestrogen receptors in amounts very similar to that of the normal littermates. 相似文献
AbstractExperimental conditions for the optimal measurement of estrogen (ER) and progesterone (PR) receptors in normal vervet monkey (Cercopithecus aethiops pygerythrus) uteri are described. The uteri of this primate were found to contain relatively high concentrations of both ER and PR. Levels of ER ranged from 151 to 822 femtomoles per mg protein (mean for group assayed is 327±165 femtomoles per mg protein). PR assays were performed on the same cytosols and the levels ranged from 444 to 2267 femtomoles per mg protein (mean of 1285±511 femtomoles per mg protein). Mean Kd values for the ER- and PR-ligand complexes were found to be 3.15±1.4x10-10 M and 2.38±0.2x10-9 M respectively, within the group analysed (n=21). The ratio of PR to ER varied between 1.1 and 13.1 with a mean of 4.5±2.4. Ligand specificity studies revealed that [3H]-17β-estradiol binding to the ER could only be inhibited by estrogens or estrogen analogues. The PR however exhibited an affinity for a wider range of ligand types. In low ionic strength buffers both ER and PR sedimented as ±8S type molecules in the presence or absence of 10mM sodium molybdate. Both receptors dissociated into smaller components, following a short exposure to 0.4 M KCl and subsequent centrifugation in a gradient containing 0.4 M KCl. 相似文献
Cytosol preparations of fat bodies from adult Leucophaea maderae contained a population of very high affinity JH binding compounds (Kd of 10−9 M) which was only identifiable by the dextrancoated charcoal assay. These compounds exhibited a 1.5 times higher affinity to the natural enantiomer (10R-JH III) than to the racemate. A binding compound for JH III with similar affinity and identical sedimentation characteristics on sucrose gradients could be extracted from isolated nuclei of only vitellogenic fat bodies, either natural or (RS)-methoprene induced. This high affinity JH binder could not be extracted from nuclei of fat bodies from males except those males which had been treated with the JH analogue. These same males were induced to synthesize vitellogenin. A population of lower affinity JH binders (Kd of 10−8 M) was identified in cytosol and nuclear extracts by the DCC assay procedure as well as by the polyethylene glycol and hydroxylapatite assays. We conclude that the high affinity JH binder of cytosol and nuclei of fat bodies is the JH receptor of this species. 相似文献
Appropriate methods for repeated surgical collection of endometrial tissue from rhesus monkeys, and characterization of cytosol and nuclear estrogen (E2) and progesterone (P) receptors (R) are described. Tissue collection was made in the mid-luteal phase at abdominal fundal hysterotomy. Functional status of the ovaries was determined by visual inspection and RIA of E2 and P in serum. Receptor assay procedures were devised permitting the measurement of total cytosol and nuclear receptor concentration. Sucrose density gradients of labelled cytosol were made and a 4S saturable binding component for 3H P and for 3H E2 were found. Equilibrium dissociation constants of 3H E2 and 3H R5020 were 2.1×10?10M and 3.6 × 10?9M, respectively. These binding characteristics are similar to those found in human endometrium and suggest that these surrogate primates have extensive utility in investigation of factors influencing E2R and PR concentrations in endometrial tissue during the menstrual cycle and implantation. Simulated menstrual cycle were produced in 20 castrate monkeys by sequential treatment with estradiol and progesterone in silastic capsules. RIA of E2 and P, and gonadotropins in peripheral serum provided assuredness of the hormonal status of each monkey under treatment. Cytosol and nuclear receptors for E2 and P were measured in the endometrium after different intervals of the treatment. E2 receptor (E2R) levels were not changed during the estrogen sequence, but were lowered by progesterone therapy in both cytosol and nuclear components. Progesterone receptor (PR) synthesis in cytosol was induced by exogenous estrogen. The total concentration of PR decreased with the uptake of P by the cell; meanwhile, the ratio of cytosol to nuclear P receptors declined. These data suggest that this sequential estrogen-progesterone regimen induces the changes in E2R and PR patterns in the endometrium of ovariectomized monkeys which occurs due to ovarian cyclicity in the normal menstrual cycle. 相似文献
Complex formation between Pd(II), Pt(II) and iodide has been studied at 25 °C for an aqueous 1.00 M perchloric acid medium. Measurements of the solubility of PdI2(s) in aqueous mercury(II) perchlorate and of AgI(s) and PdI2(s) in aqueous solutions of Pd2+(aq) and Ag+(aq) gave the solubility product of PdI2(s) as Kso=(7±3) × 10−32 M3, which is much smaller than previous literature values.The stability constants β1=[MI(H2O)3+]/([M(H2O)42+][I−]) for the two systems were obtained as the ratio between rate constants for the forward and reverse reactions of (i). The following values of k1 (s−1 M−1), k−1 (s−1) and β1 (M−1) were obtained at 25 °C: (1.14±0.11) × 106, (0.92±0.18), (12±4) × 105 for MPd, and (7.7±0.4), (8.0±0.7) × 10−5, (9.6±1.3) × 104 for MPt. Combination with previous literature data gives the following values of log(β1 (M−1)) to log(β4 (M−4)): 6.08, ∼22, 25.8 and 28.3 for MPd, and 4.98, ∼25, ∼28, and ∼30 for MPt. The present results show that the large overall stability constants β4 observed for the M2+I− systems are most likely due to a very large stability of the second complex MI2(H2O)2, which is probably a cis-isomer. A distinct plateau in the formation curve for mean ligand number 2 is obtained both for MPd and Pt. The other iodo complexes are not especially stable compared to those of chloride and bromide.ΔH≠ (kJ mol−1) and ΔS≠ (JK−1 mol−1) for the forward reaction of (i), MPd, are (17.3±1.7) and (−71±5), and for the reverse reaction of (i) MPd, (45±3) and (−95±6), respectively. The kinetics are compatible with associative activation (Ia). The contribution from bond-breaking in the formation of the transition state seems to be less important for Pd than for Pt. 相似文献
Specific binding sites for vasoactive intestinal peptide (VIP), a potent vasodilatory polypeptide, and its effect on formation of intracellular cyclic AMP levels were studied in cultured vascular smooth muscle cells (VSMC) from rat aorta. Specific binding of 125I-labeled-VIP to cultured VSMCs was time- and temperature-dependent. Scatchard analysis of binding studies suggested the presence of two classes of high and low affinity binding sites for VIP; the apparent Kd and the number of maximal binding capacity were ∼8×10−9 M and 60,000 sites/cell (high-affinity sites) and ∼4×10−8 M and 140,000 sites/cells (low-affinity sites), respectively. Unlabeled VIP competitively inhibited the binding of 125I-labeled-VIP to its binding sites, whereas neither peptides structurally related to VIP, nor other vasoactive substances affected the binding. VIP stimulated formation of intracellular cyclic AMP in cultured VSMCs in a dose-dependent manner; the stimulatory effect of VIP on cyclic AMP formation was not blocked by propranolol and was additive with isoproterenol. The present study first demonstrates the presence of specific receptors for VIP in VSMCs functionally coupled to adenylate cyclase system. It is suggested that VIP exerts its vasodilatory effect through its specific receptors distinct from β-adrenergic receptors. 相似文献
The reaction of 2,3-tri with CrCl3·6H2O1, dehydrated in boiling DMF, results in the formation of mer-CrCl3(2,3-tri) and anation of hydrolysed solutions of mer-MCl3(2,3,-tri) (M=Co, Cr) with 6 M HCl containing HClO4, forms trans-dichloro- mer-[MCl2(2,3-tri)(OH2)]ClO4·H2O (M=Cr, Co; I, II). trans-Dinitro-mer-[Co(NO2)2(NH3)(2,3-tri)] ClO4 crystallises from the reaction between mer-Co(NO2)3(2,3-tri) and aqueous 7 M ammonia, on addition of NaClO4·H2O, and trans-dichloro-mer-[CoCl2(NH3)(2,3-tri)]ClO4 (III) can be isolated by treatment of the dinitro with 12 M HCl. Reaction of mer-CoCl3(2,3-tri) with C2O42−, followed by addition of aqueous NH3 and NaClO4·H2O results in the isolation of racemic mer-[Co(ox)(NH3)(2,3-tri)]ClO4· H2O. This complex was resolved into its enantiomeric forms and treatment of these with SOCl2/MeOH/ HClO4 gave the chiral forms of trans-dichloro-mer- [CoCl2(NH3)(2,3-tri)]ClO4 (R or S at the see-NH center). The rates of loss of the first chloro ligand from these dichloro complexes have been measured spectrophotometrically in 0.1 M HNO3 over a 15 K temperature range to give the following kinetic parameters; (I) kH(298)=7.25 × 10−5 s−1, Ea=78.5 kJ mol−1, δS298#=−69 J K−1 mol−1; (II) kH(298)=4.00 × 10−3 s−1, Ea=89.9, δS298#= +87.5; (III) kH(298)=3.09 × 10−4 s−1, Ea=103, δS298#=+27. Treatment of the dichloro cations with Hg2+/HNO3 results in the generation of mer- M(2,3-tri)(OH2)33+ (M=Cr, Co; IV, V) and trans- diaqua-mer-Co(NH3)(2,3-tri)(OH2)23+ (VI). The Co(III) cations isomerise to the fac configuration with (V) Kisom(298) μ=1.0 M)=2.97 × 10−5 s−1, Ea=115, δS298#=+46. (VI) Kisom(298) (μ=1.0 M)=4.13 × 10−5 s−1, Ea=113, δS298#=+52. 相似文献
Receptors for luteinizing hormone/human chorionic gonadotropin (LH/hCG) have been identified in porcine, rabbit, rat, and human myometrium. To determine the estrous cycle and pregnancy related changes in the receptor capacity and affinity, radioreceptor assays were performed with membrane homogenates of porcine uterine tissues. Cycling gilts were divided into four experimental groups: I (n=6), day 1–2; II (n=5), day 6–7; III (n=5), day 11–12; and IV (n=6), day 18–20 of the estrous cycle. Pregnant pigs were divided into three experimental groups: I (n=5), day 35–40; II (n=5), day 65–70; and III (n=4), day 95–105 of pregnancy. The concentrations [femtomoles/mg protein (fmol/mg protein)] and affinities of unoccupied LH/hCG binding sites were characterized in all samples of myometrium. Receptor concentrations were highest (P<0.01) in groups II and III (19.3±2.5 and 35.8±2.1 fmol/mg protein, respectively), and was lowest in groups I and IV (5.3±1.4 and 7.5±0.7 fmol/mg protein, respectively). Receptor affinity constants (Ka) were consistent (P>0.05) throughout the estrous cycle [I, (5.1±1.5)×109; II, (3.0±0.8)×109; III, (3.2±0.9)×109; IV, 5.5±0.7×109 lm−1]. Plasma hormone concentrations of progesterone, estrogen and LH were typical of values noted at these times. During pregnancy, receptor concentrations were greatest (P<0.05) in group II (85.4±18.5 fmol/mg protein). In groups I and III receptor numbers were 10.8±2.3 and 26.7±6.6 fmol/mg protein, respectively. The Ka in group I was 10 times greater (P<0.05) than Ka in groups II and III, (I, 3.1±0.9×1010 lm−1; II, 3.4±0.3×109 lm−1; III, 3.3±1.1×109 lm−1). Plasma hormone concentrations typically found during pregnancy were noted. The function of these LH/hCG binding sites remains unknown; however, changes in receptor capacity during the estrous cycle and pregnancy support a role for modulation of the receptor by hormonal factors. 相似文献
1. Sitophilus oryzae (Curculionidae) and Palembus dermetoides (Tenebrionidae) esterases were studied to determine the correlation between in vitro esterase inhibition and in vivo toxicity of several insecticides.2. Km values for S. oryzae and P. dermetoides were 0.118 mM and 0.087 mM respectively.3. In vitro esterase inhibition by organophosphates and carbamates showed that for S. oryzae dichlorvos (I50 = 7 × 10−6 M) and eserine sulphate (I50 = 5 × 10−5 M) were most potent; for P. dermestoides it was methomyl (I50 = 2.8 × 10−7 M) and dichlorvos (I50 = 10−6 M). For both species chlorpyrifos-methyl was least so.4. Only slight correlation between in vitro esterase inhibition and in vivo toxicity of the insecticides could be shown for either species. This is discussed. 相似文献
The different murine D2-type dopamine receptors (D2L, D2S, D3L, D3S, and D4) were expressed in Xenopus laevis oocytes. The D2-type receptors were all similarly and efficiently expressed in Xenopus oocytes and were shown to bind the D2 antagonist [125I]sulpride. They were all shown to activate Cl− influx upon agonist stimulation. Using the diagnostic inhibitor bumetanide, we were able to separate the Na+/K+/2Cl− cotransporter component of the Cl− influx from the total unidirectional Cl− influx. The D3L subtype was found to operate exclusively through the bumetanide-insensitive Cl− influx whereas the other D2-type receptors acted on the Na+/K+/2Cl− cotransporter as well. The pertussis toxin sensitivity of the receptor-activated chloride influx via the Na+/K+/2Cl− cotransporter varied between the various D2-type receptors showing that they may couple to different G proteins, and activate different second messenger systems. 相似文献
The present study investigates the effect of a partially purified thymus factor, thymosin Fraction 5, and an homogeneous polypeptide component of Fraction 5, thymosin α1, on glucocorticoid resistance and glucocorticoid receptors in mouse thymocytes. Treatment of thymocytes in vitro with thymosin Fraction 5 or α1, results in an increase in the percentage of glucocorticoid-resistant cells. Studies on the specific whole-cell binding of [3H]dexamethasone and steroid competition experiments demonstrate the existence of high-affinity (Kd = 1.0 × 10?8M) specific glucocorticoid receptors in mouse thymocytes. Preincubation with thymosin Fraction 5 or α1 appears to cause a reduction in the specific [3H]dexamethasone binding to intact thymocytes. 相似文献
A membrane-bound (nitrate, chloride)-activated AT Pase was found in the neritie diatom, Skeletonema costatum (Grev.) Cleve. The enzyme is suggested to translocate NO3− across the plasmalemma, against a concentration gradient. The Km of the enzyme with respect to NO3− is ca. 0.9 × 10−6 M, and is in close agreement with the reported K8 for NO3− uptake by the whole cell. 相似文献
A kinetic study of the oxidation of (hydroxyethyl)ferrocene (HEF) by [2-pyridylmethylbis(2-ethyl-thioethyl)ainine]copper(II) (Cu(pmas)2+) is reported, with the objective of documenting the influence of the two thioether sulfur ligands on the electron transfer rate. Both reactants exhibit a first-order dependence at pH 6, I = 0.1 M(NaNO3); k(25°C) = 1.3 × 104M−1sec−1, ΔH3 = 10.1 kcal/mole, ΔS3 = −6 eu. The apparent Cu(pmas)2+/+ self-exchange electron transfer rate constant calculated from this reaction on the basis of relative Marcus theory (4.7 × 101M−1 sec−1) agrees well with previous findings on ferrocytochrome c, Fe(CN)64−, and Ru(NH3)5py2+ oxidations. Spectrophotometric titrations of Cu(pmas)2+ and Cu(tmpa)2+ (tmpa = tris(2-pyridylmethyl)amine) with azide ion showed that both Cu(pmas)N3)+ (Kf1 = 3.1 × 103M−1) and Cu(pmas)(N3)2 (Kf2 = 3.5 × 101M−1) but Cu(tmpa)(N3)+ (Kf = 6.6 × 102M−1) are formed up to 0.15 M N3− (25°C, pH 6, I = 0.2 M), suggesting that a thioether sulfur atom is displaced in the uptake of a second N3− ion by Cu(pmas)(N3)+. The effect of thioether sulfur displacement by azide ion on the HEF-Cu(pmas)2+ reaction rate may be understood entirely through the tendency of N3− to shift the position of the redox equilibrium towards the reactant side, without invoking any special role for the sulfur ligand in promoting electron transfer reactivity. 相似文献
Quantitative analyses of LH-RH-like membrane receptors were performed in five tumors from the transplantable Dunning R3372H rat prostatic adenocarcinoma. The binding of D-Trp6-LH-RH, an agonist of LH-RH, was observed in all 5 tumors. The antagonist [Ac-Dp-Cl-Phe1,2,D-Trp3,D-Lys6,D-Ala10]-LH-RH was bound to 4 tumors. The apparent equilibrium dissociation constant (Kd) for D-Trp6-LH-RH receptor was from 2.6–3.9 × 10?10 M. The apparent equilibrium Bmax values (maximum number of binding sites) were from 17.2–86.0 fmol/mg membrane protein for D-Trp6-LH-RH receptor. The Kd for the antagonist was from 2.4–2.7 × 10?10 M and the Bmax values were from 35.5–66.0 fmol/mg membrane protein. Similar binding studies performed in 6 normal rat prostates showed no binding capacities. 相似文献
