Kinetics of active and passive components of water exchange between the air and a mite, Dermatophagoides farinae

Female North American house dust mites were found to exchange water with the ambient air from two compartments. At humidities above the critical equilibrium activity (CEA), transpiration out of a single large compartment was observed using HTO as a tracer for water. Total sorption into this compartment was also observed by following changes in the specific radioactivity. The sorption data required that an active process or pump be present. The water in this pump is the second compartment above the CEA. Below the CEA the large compartment could be identified as a compartment characterized by a small transpiration rate constant. The pump below the CEA becomes a rapidly transpiring fast compartment. By separating the water pool into two compartments, it was possible to relate a_v to k and $\text{m}\text{?}{}_{\mathrm{<mtext>S</mtext>}}$. The major effect of a_v on k was related to its effect on the permeability of the cuticle. The influence of a_v on $\text{m}\text{?}{}_{\mathrm{<mtext>S</mtext>}}$ was different for active and passive sorption. Above the CEA the pump operated at full capacity and active $\text{m}\text{?}{}_{\mathrm{<mtext>S</mtext>}}$ was directly proportional to a_v. Passive sorption was influenced by a_v in two ways. The driving force for $\text{m}\text{?}{}_{\mathrm{<mtext>S</mtext>}}$ was further reduced below saturation by the effect of a_v on the permeability of the exchange surface.     

Tests of the carrier model for ion transport by nonactin and trinactin

The fluxes of K⁺ and NH₄⁺ carried by nonactin and trinactin across thin lipid membranes have been measured as functions of ion activity, electric potential and time. In agreement with the predictions of a version of the carrier model in common use, the shape of the initial current-voltage relation is independent of the activity of the electrolyte, $\text{a}{}_{\mathrm{<mtext>i</mtext>}}$ while the ratio of the initial conductance, $\text{G}{}_0$, to the steady-state conductance, $\text{G}{}_{\mathrm{\infty }}$, increases according to $\text{G}{}_0\text{/G}{}_{\mathrm{\infty }}\text{=}\text{const}{}_1\text{+ const}{}_2\text{× a}{}_{\mathrm{<mtext>i</mtext>}}$. For trinactin the data presented allow the estimation of the rate constants of the carrier process (in the limit of zero potential) in a manner which does not assume any particular variation with potential for the constants. Using empirically determined functions of potential, a complete set of values is also available for nonactin. The curve fitting which is necessary is described in the following paper. The data presently available for valinomycin are sufficient neither to test the model nor to determine a complete set of constants.     

Equilibrium constants under physiological conditions for the reactions of L-phosphoserine phosphatase and pyrophosphate: L-serine phosphotransferase

The observed equilibrium constants (K_obs) for the l-phosphoserine phosphatase reaction [EC 3.1.3.3] have been determined under physiological conditions of temperature (38 °C) and ionic strength (0.25 m) and physiological ranges of pH and free [Mg²⁺]. Using Σ and square brackets to indicate total concentrations $\text{K}{}_{\mathrm{<mtext>obs</mtext>}}\text{=}\text{Σ L-serine][Σ P}{}_{\mathrm{i}}\text{]}\text{Σ L-phosphoserine]H}{}_2\text{O]}\text{, K =}\text{L-H · serine}{}^{\mathrm{\pm }}\text{]HPO}{}_4{}^{\mathrm{2?}}\text{]}\text{[L-H · phosphoserine}{}^{\mathrm{2?}}\text{]H}{}_2\text{O]}$. The value of K_obs has been found to be relatively sensitive to pH. At 38 °C, K⁺] = 0.2 m and free [Mg²⁺] = 0; K_obs = 80.6 m at pH 6.5, 52.7 m at pH 7.0 [ΔG_obs⁰ = ?10.2 kJ/mol (?2.45 kcal/mol)], and 44.0 m at pH 8.0 ([H₂O] = 1). The effect of the free [Mg²⁺] on K_obs was relatively slight; at pH 7.0 ([K⁺] = 0.2 m) K_obs = 52.0 m at free [Mg²⁺] = 10^?3, m and 47.8 m at free [Mg²⁺] = 10^?2, m. K_obs was insignificantly affected by variations in ionic strength (0.12–1.0 m) or temperature (4–43 °C) at pH 7.0. The value of K at 38 °C and I = 0.25 m has been calculated to be 34.2 ± 0.5 m [ΔG_obs⁰ = ?9.12 kJ/mol (?2.18 kcal/ mol)]([H₂O] = 1). The K for the phosphoserine phosphatase reaction has been combined with the K for the reaction of inorganic pyrophosphatase [EC 3.6.1.1] previously estimated under the same physiological conditions to calculate a value of 2.04 × 10⁴, m [ΔG_obs⁰ = ?28.0 kJ/mol (?6.69 kcal/mol)] for the K of the pyrophosphate:l-serine phosphotransferase [EC 2.7.1.80] reaction. $\text{K}{}_{\mathrm{<mtext>obs</mtext>}}\text{=}\text{[}\text{Σ L-serine}\text{][}\text{Σ}\text{P}{}_{\mathrm{<mtext>i</mtext>}}\text{]}\text{[}\text{Σ L-phosphoserine}\text{][}\text{H}{}_2\text{O}\text{]}\text{, K =}\text{[L-H · serine}{}^{\mathrm{\pm }}\text{]HPO}{}_4{}^{\mathrm{2?}}\text{]}\text{[L-H · phosphoserine}{}^{\mathrm{2?}}\text{]H}{}_2\text{O}$. Values of K_obs for this reaction at 38 °C, pH 7.0, and I = 0.25 m are very sensitive to the free [Mg²⁺], being calculated to be 668 [ΔG_obs⁰ = ?16.8 kJ/mol (?4.02 kcal/mol)] at free [Mg²⁺] = 0; 111 [ΔG_obs⁰ = ?12.2 kJ/mol (?2.91 kcal/mol)] at free [Mg²⁺] = 10^?3, m; and 9.1 [ΔG_obs⁰ = ?5.7 kJ/mol (?1.4 kcal/mol) at free [Mg²⁺] = 10^?2, m). K_obs for this reaction is also sensitive to pH. At pH 8.0 the corresponding values of K_obs are 4000 [ΔG_obs⁰ = ?21.4 kJ/mol (?5.12 kcal/mol)] at free [Mg²⁺] = 0; and 97.4 [ΔG_obs⁰ = ?11.8 kJ/ mol (?2.83 kcal/mol)] at free [Mg²⁺] = 10^?3, m. Combining K_obs for the l-phosphoserine phosphatase reaction with K_obs for the reactions of d-3-phosphoglycerate dehydrogenase [EC 1.1.1.95] and l-phosphoserine aminotransferase [EC 2.6.1.52] previously determined under the same physiological conditions has allowed the calculation of K_obs for the overall biosynthesis of l-serine from d-3-phosphoglycerate. $\text{K}{}_{\mathrm{<mtext>obs</mtext>}}\text{=}\text{[}\text{Σ L-serine}\text{][}\text{Σ NADH}\text{][}\text{Σ}\text{P}{}_{\mathrm{<mtext>i</mtext>}}\text{][}\text{Σ}\text{α-}\text{ketoglutarate}\text{]}\text{[Σ d-3-}\text{phosphoglycerate}\text{][Σ NAD}{}^{\mathrm{+}}\text{][Σ L-glutamat0]}$ The value of K_obs for these combined reactions at 38 °C, pH 7.0, and I = 0.25 m (K⁺ as the monovalent cation) is 1.34 × 10^?2, m at free [Mg²⁺] = 0 and 1.27 × 10^?2, m at free [Mg²⁺] = 10^?3, m.     

The cell cycle time of the haemocytes in the insect Calliphora vicina

The cell cycle time of Calliphora vicina prohaemocytes was examined using the labelled mitoses method after the administration of a pulse of H³-thymidine. The total cycle time occupied 9.1 hr, while $\text{G}{}_1\text{+}\text{1}\text{2}\text{M}$, S and $\text{G}{}_2\text{+}\text{1}\text{2}\text{M}$ occupied 1.6 hr, 2.7 hr and 4.8 hr respectively.     

Stereochemical control of yeast reductions. 2. Quantitative treatment of the kinetics of competing enzyme systems for a single substrate

Quantitative expressions have been developed for systems such as yeast reductions where competing enzymes act on one substrate to yield two enantiomeric products. These expressions relate the observed stereochemical variables, the extent of conversion (C), the optical purity expressed as enantiomeric excess (ee), and the initial substrate concentration (A₀) to the kinetic parameters K_R and K_S (apparent Michaelis constants) and y ($\text{V}{}_{\mathrm{R}}\text{V}{}_{\mathrm{S}}$, the ratio of maximal velocities) of such competing enzymes. The expressions have been experimentally verified using a purified competing enzyme system of l- and d-lactic dehydrogenases. Furthermore, the enantioselective reduction of β-keto esters by intact yeast cells has been examined by means of this kinetic analysis.     

Time lag in a model of a biochemical reaction sequence with end product inhibition

The model studied is that of Goodwin, in which all but one of the reactions obey linear kinetics, while the end-product inhibits the first reaction in a term of Michaelis-Menten form, with Hill coefficient ?:

$\text{z=}\text{∫}\text{?∞}\text{t}\text{x}{}_{\mathrm{n}}\text{(T)G(t?T)dt}$

The results obtained relate to time lag in the off diagonal terms in these equations. The time lag is taken in distributed form, for example replacing x_n in the first equation by

$\text{dx}{}_{\mathrm{t}}\text{dt}\text{=k}{}_1\text{x}{}_{\mathrm{t??}}\text{1?b}{}_1\text{x}{}_{\mathrm{t}}\text{, i=2, …n.}$

For any non-negative G, time lag in these terms can not destabilize the equilibrium point in the case ? = 1. For a particular class of functions G one can obtain some insight into the consequences of time lag by relating the model to that with a longer loop of reactions. Then known results can be used for general ? and n.     

The effect of multiple inseminations on the evolution of social behaviors in diploid and haplo-diploid organisms

Using a classical population genetic model, the necessary conditions for the spread of genes that determine social behaviors and the rate of spread of these genes are derived. The influence of 1, 2, 3, or k inseminations per female on these conditions is investigated for both diploid and haplodiploid organisms. These results are then extended to a population in which there are arbitrary variations among females in their numbers of mates. These results do not depend upon assuming equal paternity by all inseminating males; the effects of sperm competition and unequal paternity are also derived. The rates and conditions for social evolution in these groups of complex composition are discussed in relation to Hamilton's rule.For all models, the total change in gene frequency, Δq, is partitioned into two components: (1) $\text{Δq}{}_{\mathrm{I}}$, the change in gene frequency caused by selection within groups; this component is always negative, illustrating that individual selection always operates against the evolution of social behaviors; and (2) Δq_G, the change in gene frequency caused by selection between groups; this component is generally positive. Hamilton's rule is shown to specify the necessary and sufficient conditions for $\text{Δq}{}_{\mathrm{G}}\text{> |}\text{Δq}{}_{\mathrm{I}}\text{|}$, that is, for selection among kin groups to over-ride individual selection within kin groups.     

Catalytic function of thymidylate synthase is confined to S phase due to its association with replitase

Catalytic activity of thymidylate synthase, as measured $\text{in}\text{,}\text{vivo}$, is tightly linked to S phase of the cell cycle in Chinese hamster embryo fibroblast cells. This activity, as measured $\text{in}\text{,}\text{vitro}$, is found in all parts of the cell cycle. Thymidylate synthase activity in nuclear (karyoplast) extracts increased as the cells progressed from $\text{G}{}_0\text{G}{}_1$ to S phase. This enzymatic activity in the nuclei of S phase cells is associated with the multienzyme complex (replitase) that also contained DNA polymerase and other enzymes of DNA replication and precursor synthesis. The degree of association of thymidylate synthase with replitase, which increased co-ordinately as the cells progressed from $\text{G}{}_0\text{G}{}_1$ phase to S phase, coincided strongly with the level of $\text{in}\text{,}\text{vivo}$ activity of the enzyme.     

Interaction of lymphocytes and macrophage cell line cells (M1 cells). I. Functional maturation and appearance of Fc receptors im M1 cells

M₁ cells, which are cell line cells established from myeloid leukemia cells of the SL strain mouse, can differentiate from blast cells ($\text{M}{}_1{}^{\mathrm{?}}$) to mature macrophages ($\text{M}{}_1{}^{\mathrm{+}}$) within 48 hr, when they are cultured with conditioned medium (CM) obtained from murine embryonic fibroblasts. While $\text{M}{}_1{}^{\mathrm{?}}$ cells have no phagocytic activity nor Fc receptor (FcR), $\text{M}{}_1{}^{\mathrm{+}}$ cells possess both characteristics. The appearance of FcR is temperature-dependent and inhibited by a metabolic inhibitor, cycloheximide. FcR on $\text{M}{}_1{}^{\mathrm{+}}$ cells is resistant to trypsin and pronase. $\text{M}{}_1{}^{\mathrm{+}}$ cells improve the viability of macrophage-depleted SL splenic lymphocytes and restore the in vitro secondary plaque forming cell response of macrophage-depleted spleen cells to particulate and soluble antigens. $\text{M}{}_1{}^{\mathrm{?}}$ cells lack this macrophage-substituting capacity. Mm₁ cells, mutant cells from M₁ cells, having FcR and higher phagocytic activity than $\text{M}{}_1{}^{\mathrm{+}}$ cells, are also devoid of this capacity.     

Deoxyribose 5-phosphate aldolase: an enzyme that peaks in the G2 phase of rat hepatoma cells.

The activity of deoxyribose 5-P aldolase (2-deoxy-d-ribose 5-phosphate acetaldehyde lyase, EC 4.1.2.4) increases three- to fourfold in cultures of rat hepatoma cells that have reached stationary growth and have stopped in the G₂ phase of the cell cycle. We have shown that in cell cultures synchronized by three independent methods the enzyme activity peaks in late G₂, followed by a rapid decline during mitosis. Two compounds, dibutyryl cAMP and isoproterenol, that appear to block these cells in G₂, also cause a two- to fourfold increase in deoxyribose 5-P aldolase activity. It is suggested that this enzyme may play a role in lowering the pools of deoxyribonucleotides in the late $\text{G}{}_2\text{M}$ phase of the cell cycle.     

A convective mass transfer model for determining intestinal wall permeabilities: laminar flow in a circular tube

A convective mass transfer model as analyzed and developed for use in determining intestinal wall permeabilities from external perfusion experiments. Analysis of the model indicates that the ratio of the exit to inlet concentration $\text{C}{}_{\mathrm{m}}\text{C}{}_0$ is a function of only two dimensionless independent variables, the wall permeability, $\text{P}{}_{\mathrm{w}}{}^1$ and Graetz number, Gz = πDL/2Q. The Graetz number contains the independent variables of interest, length, diflusivity, and flow rate. The radius of the intestine is included implicitly in the flow rate. Since $\text{C}{}_{\mathrm{m}}\text{C}{}_0$ and Gz are the experimental quantities, and the solution to the model system contains P_ω¹ implicitly, a convenient approximate method is developed which allows a direct calculation of P_ω¹. This method is in error by 10–20% in the worst cases. The approach is illustrated by application to the determination of the wall permeabilities for two non polar compounds.     

Stimulation of DNA synthesis and cell division in a chemically defined medium: Effect of Epidermal Growth Factor,Insulin and Vitamin B12 on resting cultures of 3T6 cells

Addition of Epidermal Growth Factor, Insulin and Vitamin B₁₂ in completely serum free medium to cultures of 3T6 cells arrested in the $\text{G}{}_1\text{G}{}_0$ phase of the cell cycle stimulates DNA synthesis in 80–90% of the cell population. Cell division occurs 48–72 hours after factor addition. Because the peptides are active at low levels and interact synergistically, this model system offers a powerful tool for elucidating mechanisms of growth regulation which might have a physiological relevance.     

Oxidative phosphorylation by membrane vesicles from Bacillus alcalophilus

ADP and P_i-loaded membrane vesicles from l-malate-grown Bacillus alcalophilus synthesized ATP upon energization with $\text{ascorbate}\text{N,N,N′,N′-}\text{tetramethyl}\text{-p-}\text{phenylenediamine}$. ATP synthesis occurred over a range of external pH from 6.0 to 11.0, under conditions in which the total protonmotive force was as low as ?30 mV. The phosphate potentials (ΔG_p) were calculated to be 11 and 12 kcal/mol at pH 10.5 and 9.0, respectively, whereas the values in vesicles at these two pH values were quite different (?40 ± 20 mV at pH 10.5 and ?125 ± 20 mV at pH 9.0). ATP synthesis was inhibited by KCN, gramicidin, and by N,N′-dicyclohexylcarbodiimide. Inward translocation of protons, concomitant with ATP synthesis, was demonstrated using direct pH monitoring and fluorescence methods. No dependence upon the presence of Na⁺ or K⁺ was found. Thus, ATP synthesis in B. alcalophilus appears to involve a proton-translocating ATPase which functions at low .     

Involvement of thyroid gland in the development of migratory disposition in the redheaded bunting, Emberiza bruniceps

In the redheaded bunting Emberiza bruniceps, thyroidectomy inhibited premigratory fattening and nocturnal restlessness—two characteristics of avian migration—observed in caged birds during the premigratory period (March/April). Thyroxine (T₄) and triiodothyronine (T₃) administration in thyroidectomized birds stimulated locomotor activity and restored the loss in body weight. Annual variations in circulating thyroid hormone concentrations revealed a significant rise in $\text{T}{}_3\text{T}{}_4$ ratio prior to spring migration in both years studied. This increase in circulating $\text{T}{}_3\text{T}{}_4$ ratio may be associated with the development of migratory disposition in this bird. There was no increase in circulating $\text{T}{}_3\text{T}{}_4$ ratio prior to autumnal migration, however, plasma T₄ increased significantly. Different thyroidal mechanisms are most likely involved in spring and fall migratory periods. While T₃ remained low throughout, apart from the characteristic spring rise, high T₄ levels in E. bruniceps were associated with periods of reproduction and molting, the latter coinciding partly with autumnal migration.     

Effects of 5-hydroxylysine on acetylene reduction and NH4+-assimilation in the cyanobacterium Anabaena cylindrica.

5-hydroxylysine, an analogue of glutamate and lysine, causes $\text{NH}{}_4{}^{\mathrm{+}}$ production by N₂-fixing A. cylindrica; it also reversibly inhibits GS activity in vitro but has no effect on alanine dehydrogenase or GOGAT. On adding 5-hydroxylysine intracellular pools of glutamine, glutamate and aspartate decrease; those of alanine and serine increase. 5-hydroxylysine alleviates the inhibitory effect of $\text{NH}{}_4{}^{\mathrm{+}}$ on heterocyst production and C₂H₂ reduction and in $\text{NH}{}_4{}^{\mathrm{+}}\text{-grown}$ cultures results in heterocyst synthesis and in C₂H₂ reduction. The data suggest that the GS-GOGAT pathway is the sole route of importance in primary $\text{NH}{}_4{}^{\mathrm{+}}$ assimilation in A. cylindrica, that $\text{NH}{}_4{}^{\mathrm{+}}$ alone does not inhibit nitrogenase and heterocyst production, and that GS and/or a product is involved in regulating the production of both.