Paramagnetic behaviour of the differentiating reproductive apex of wheat

Summary A study of the physiological significance of EPR signal was undertaken in the developing apical organs as well as in the top most leaf of a determinate type of plant,Triticum aestivum Cv. S 227 at various stages of vegetative and reproductive differentiation. Pour types of signals are reported: (a) a weak asymmetrical signal having 700 Gauss of width and g=2, the origin of which, is not clear; (b) a broad six peak signal also having g=2 which, as available evidence suggests, may be due to Mn⁺⁺; (c) in association with Mn⁺⁺ signal there are also other signals caused either by paramagnetic metals or by organic free radicals (FR); (d) at the centre of Mn⁺⁺ signal there appears a free radical signal with g=2.0023. It is observed that the amplitude of Mn⁺⁺ and free radical signal increases sharply in the shoot apex during its transformation from vegetative to reproductive state. The leaf also consistently records higher Mn⁺⁺ and FR contents at all stages of reproductive differentiation. Synchronously with the above mentioned enhanced paramagnetic behaviour of the apex and of the leaf there is an upsurge in metabolic activity of the plant. The possible role of free radicals and Mn⁺⁺ in energy transfer is discussed in relation to ascorbic acid turnover.     

The Importance of Calcium in Poststimulation Potentiation

Isotonic contractions recorded both before and during poststimulation potentiation in the toad isolated ventricle (Bufo marinus) revealed that the phenomenon of poststimulation potentiation was not altered by the presence or absence of the catechol amines, or by the specific amine antagonist, DCI. Similarly the inhibitors, sodium fluoride and sodium iodoacetate, were without effect. Changes in [Ca⁺⁺], [Mg⁺⁺], and [Na⁺] affected the degree of potentiation. High [Ca⁺⁺] as well as the cardiac glycosides abolished it, low [Na⁺] and the absence of Mg⁺⁺ depressed it. It has been shown that the percentage potentiation depends to some extent upon the total number of contractions occurring during the rapid stimulation phase. The amplitude of the contractions during this stage did not influence the degree of potentiation. These results are discussed in terms of Ca⁺⁺ accumulation or redistribution associated with an early phase of the membrane depolarization.     

Influence of carbon dioxide enrichment, ozone and nitrogen fertilization on cotton (Gossypium hirsutum L.) leaf and root composition

The objective of this study was to test whether elevated [CO₂], [O₃] and nitrogen (N) fertility altered leaf mass per area (LMPA), non‐structural carbohydrate (TNC), N, lignin (LTGA) and proanthocyanidin (PA) concentrations in cotton (Gossypium hirsutum L.) leaves and roots. Cotton was grown in 14 dm³ pots with either sufficient (0·8 g N dm ^{? 3}) or deficient (0·4 and 0·2 g N dm ^{? 3}) N fertilization, and treated in open‐top chambers with either ambient or elevated ( + 175 and + 350 μ mol mol ^{? 1}) [CO₂] in combination with either charcoal‐filtered air (CF) or non‐filtered air plus 1·5 times ambient [O₃]. At about 50 d after planting, LMPA, starch and PA concentrations in canopy leaves were as much as 51–72% higher in plants treated with elevated [CO₂] compared with plants treated with ambient [CO₂], whereas leaf N concentration was 29% lower in elevated [CO₂]‐treated plants compared with controls. None of the treatments had a major effect on LTGA concentrations on a TNC‐free mass basis. LMPA and starch levels were up to 48% lower in plants treated with elevated [O₃] and ambient [CO₂] compared with CF controls, although the elevated [O₃] effect was diminished when plants were treated concurrently with elevated [CO₂]. On a total mass basis, leaf N and PA concentrations were higher in samples treated with elevated [O₃] in ambient [CO₂], but the difference was much reduced by elevated [CO₂]. On a TNC‐free basis, however, elevated [O₃] had little effect on tissue N and PA concentrations. Fertilization treatments resulted in higher PA and lower N concentrations in tissues from the deficient N fertility treatments. The experiment showed that suppression by elevated [O₃] of LMPA and starch was largely prevented by elevated [CO₂], and that interpretation of [CO₂] and [O₃] effects should include comparisons on a TNC‐free basis. Overall, the experiment indicated that allocation to starch and PA may be related to how environmental factors affect source–sink relationships in plants, although the effects of elevated [O₃] on secondary metabolites differed in this respect.     

How is the relationship between the C4 cereal Sorghum bicolor and the C3 root hemi-parasites Striga hermonthica and Striga asiatica affected by elevated CO2?

The C₄ cereal Sorghum bicolor was grown under either ambient (350 μmol mol^?1) or elevated (700 μmol mol^?1) [CO₂] in either the presence or absence of the C₃ obligate root hemi-parasites Striga hermonthica or S. asiatica. Both uninfected and infected sorghum plants were taller and had greater biomass, photosynthetic rates, water-use efficiencies and leaf areas under elevated compared with ambient [CO₂]. There was no evidence of any downregula-tion of photosynthesis in sorghum grown at elevated [CO₂]. Biomass of infected sorghum was lower under both ambient and elevated [CO₂], and although infected plants were larger under elevated [CO₂] the relative impact of infection on host biomass was either the same (S. asiatica) or only slightly less (S. hermonthica) than under ambient [CO₂]. In contrast, biomass of S. hermonthica and S. asiatica per host was lower under elevated than ambient [CO₂], although rates of photosynthesis were higher at elevated [CO₂] and parasite stomatal conductance was not responsive to [CO₂]. Parasites emerged above-ground and flowered earlier under ambient compared with elevated [CO₂]. It appears that the mechanism(s) by which the parasites affect host growth is (are) relatively insensitive to increased atmospheric [CO₂], although the parasites themselves were adversely affected by growth at elevated [CO₂].     

The form of sodium-calcium competition at the frog myoneural junction

The times required for a steady rate of miniature end-plate potential discharge to be reached in response to changes in extracellular [K⁺], [Na⁺], and [Ca⁺⁺] have been measured. In the presence of 15 mM KCl, Ca⁺⁺ raises and Na⁺ lowers the steady-state mepp frequency; but the depressive effect on Na⁺ is not specific: Li⁺ can replace Na⁺ to a large extent. Mepp frequency has been found to depend on the ratio of [Ca_o ⁺⁺]/[Na_o ⁺]. It is assumed that in the steady state, intracellular sodium will change when extracellular sodium is changed. Because both intracellular and extracellular sodium at motor nerve endings affect acetylcholine release, it is proposed that mepp frequency depends on the ratio [Ca_o] [Na_i]²·/[Na_o]² Two models are proposed. Firstly, to account for the action of sodium and calcium a carrier is postulated for which Ca⁺⁺ and Na⁺ compete. The carrier determines a maximum level of intracellular Ca⁺⁺ far lower than predicted by the Nernst equation for Ca. Secondly, to account for activation of acetylcholine release by a small influx of Ca⁺⁺, the ions are presumed to enter the nerve ending in a two stage process through a small intermediate compartment and to act on the acetylcholine release site in this region rather than after entering directly into the cell.     

Barium modifies the concentration dependence of active potassium transport by insect midgut

Summary The rate of active K⁺ transport by the isolated lepidopteran midgut shows a rectangular hyperbolic relation to [K⁺] over the range 20 to 70mm K⁺ in the absence of any divalent cation. Addition of Ba⁺⁺ to the hemolymph (K⁺ uptake) side introduces a linear component to the concentration dependence, such that active K^– transport is decreased at [K⁺] of 55mm or less, but increased transiently at higher [K⁺]. As [Ba⁺⁺] is increased over the range 2 to 8mm the linear component increases and the saturating component decreases; in 8mm Ba⁺⁺ the concentration dependence is dominated by the linear component. The effect of Ba⁺⁺ cannot easily be accounted for by simple competition with K⁺ for basal membrane uptake sites. Similar effects might be exercised by other alkali earth cations, since the concentration dependence of active K⁺ transport possesses a substantial linear component in solutions containing 5mm Ca⁺⁺ and 5mm Mg⁺⁺ (the alkali earth metal concentrations of standard lepidopteran saline).     

Binding of calcium and zinc to the acetylcholine receptor purified from Torpedo Californica

Binding of [⁶⁵Zn⁺⁺] and [⁴⁵Ca⁺⁺] to the acetylcholine (ACh)-receptor, purified from the $\text{Torpedo}$ electric organ, was studied by equilibrium dialysis. Whereas [⁶⁵Zn⁺⁺] bound to 56 nmoles of sites per mg protein with a dissociation constant of 2.5 × 10⁻⁶M, no binding of [⁴⁵Ca⁺⁺] at concentrations up to 10⁻³M could be detected with this method. However, the binding of [acetyl-³H]choline to the receptor was blocked equally by very high Zn⁺⁺ or Ca⁺⁺ concentrations, and the K_i for this low affinity binding was 7 × 10⁻³M. The high affinity binding of [⁶⁵Zn⁺⁺] to the receptor was blocked best by Cd⁺⁺ then Co⁺⁺ and Mn⁺⁺, but least by Mg⁺⁺ and Ca⁺⁺. When the purified ACh-receptor itself was analyzed for the presence of cations by atomic absorption, it was discovered that 4.7% of its weight was due to bound Ca⁺⁺ that could not be removed even by extensive dialysis. When Ca⁺⁺-free solutions (containing 1 mM EDTA) were used during purification, 0.6% of the molecular weight of the receptor was still due to bound Ca⁺⁺. This was equivalent to 15 moles of Ca⁺⁺ for each mole of ACh bound at saturation. It is suggested that the source of this Ca⁺⁺ is endogenous, and that it is tightly bound to the ACh-receptor molecule.     

Effects of calcium ions and quinolinic acid on rat kidney mitochondrial kynurenine aminotransferase

At pH 6.4, rat kidney mitochondrial kynurenine aminotransferase activity is enhanced several-fold by the addition of CaCl₂, apparently because Ca⁺⁺ facilitates the translocation of α-ketoglutarate, one of the substrates, across the mitochondrial inner membrane. Chloride salts or Mg⁺⁺, Mn⁺⁺, Na⁺, K⁺, and NH₄⁺ did not have this effect. At pH 6.8, the enzyme activity was near maximal even without added Ca⁺⁺ but was strongly depressed by either of two calcium chelating agents, quinolinic acid (Q.A.) and ethyleneglycol-bis(β-aminoethyl ether)N,N′-tetraacetic acid (EGTA). These observations support the view that Ca⁺⁺ is involved in regulating kidney mitochondrial translocation of α-ketoglutarate and that the reported interference of polycarboxylate anion translocation by Q.A. $\text{in vivo}$ depends on the ability of that agent to chelate Ca⁺⁺.     

Interactions des ions métalliques avec le DNA. IV. Fixation de i'ion cuivrique sur le DNA

The binding of cupric ion (Cu⁺⁺) to DNA was followed by spectrophotometry, melting profiles, and hydrodynamic techniques, in 0. 1M NaClO₄ and at pH 5. 6. A small amount of Cu⁺⁺ is bound specifically to bases (about 1 Cu⁺⁺ per 20 nucleotides), in agreement with polarographic and EPR data. A preferential stabilization of G–C pairs and only a slight increase of the flexibility of the molecule were observed. In 5 × 10^?3M NaClO₄, a higher number of nonhomogeneous binding sites is found by spectrophotometry. It is concluded that at least two types of sites are available for Cu⁺⁺. The first one, where Cu⁺⁺ is chelating N₇ of purines to phosphate, is observed only at low ionic strength and destabilizes the double helix. The second exists mainly at 0, 1M or higher ionic strength. All the sites are identical and could be attributed to two successive guanine residues in the same strand. Similar behavior was found for other divalent cations, e. g., Fe⁺⁺, Mn⁺⁺, and Co⁺⁺.     

THE EFFECT OF ENVIRONMENTAL POTASSIUM AND CALCIUM CONCENTRATIONS ON THE RECOVERY OF THE ACTION POTENTIAL AND RELATED FUNCTIONS OF NERVE

1. When the Ringer''s solution applied to isolated frog sciatic nerve contains K⁺ in concentrations greater than 2 x standard, the height of the spike and of the after-potential is decreased, as is the duration of the after-potential; recovery of height and of excitability following response is delayed; degree and duration of supernormal excitability are decreased; postcathodal depression and postanodal enhancement are increased and prolonged. 2. The nerve functions just listed in general all change in the opposite direction when exposed'' to increased environmental [Ca⁺⁺]. (4.5–20 x standard) or decreased [K⁺] (0.05–0.2 x standard). The effects of decreased [Ca⁺⁺] (0.20–0.25 x standard) are indeterminate. 3. When [K⁺] and [Ca⁺⁺] are both greater than 2 x standard, whatever the ratio between the concentrations the effects characteristic of high [K⁺] eventually predominate. However, these effects, except for those involving spike height, are preceded by effects characteristic of high [Ca⁺⁺] when this cation is present in sufficient excess. 4. When [K⁺] and [Ca⁺⁺] are reduced to equal low levels (0.1–0.2 x standard), effects characteristic of low [K⁺] and high [Ca⁺⁺] are obtained. 5. The experimentally determined order of ability of the environments to produce changes characteristic of high K⁺ (which is the reverse of the order of their ability to produce changes characteristic of high [Ca⁺⁺]), is not the order of their K⁺ or Ca⁺⁺ concentrations, nor of the ratio between these concentrations (Table II). 6. The results may be explained by the assumption that the functions investigated are all to greater or less degree controlled by (1) the [K⁺]/[Ca⁺⁺] ratio and (2) the K⁺ concentration, at least when this exceeds a critical level. Control by [K⁺] is more effective for spike height and its recovery after stimulation than for the other functions. The special rôle of K⁺ is attributed to an unknown specific effect of this ion which Ca⁺⁺ is unable to oppose. It is suggested that this K⁺ effect in general becomes marked on the frog nerve functions investigated when the K⁺ concentration is somewhat above 2 x standard, while the [K⁺]/[Ca⁺⁺] ratio must be changed by a factor of 4 or more before it exerts a definite effect on these functions. 7. In standard and in modified cationic environments, nerve functions vary in the ease with which they manifest changes characteristic of high [K⁺] or of high [Ca⁺⁺]. 8. The after-potential functions are less completely controlled by the cationic environment than are the other functions investigated.     

Matrix free Mg2+ and the regulation of mitochondrial volume

Mitochondria must maintain volume homeostasis inorder to carry out oxidative phosphorylation. It has been postulatedthat the concentration of freeMg²⁺([Mg²⁺]) serves as thesensor of matrix volume and regulates aK⁺-extrudingK⁺/H⁺antiport (K. D. Garlid. J. Biol. Chem.255: 11273-11279, 1980). To test this hypothesis, the fluorescentprobe furaptra was used to monitor[Mg²⁺] and freeCa²⁺ concentration ([Ca²⁺]) in the matrix ofisolated beef heart mitochondria, andK⁺/H⁺antiport activity was measured by passive swelling in potassium acetate. Concentrations that result in 50% inhibition of maximum activity of 92 µM matrix [Mg²⁺] and 2.2 µM[Ca²⁺] were determined for theK⁺/H⁺ antiport. Untreated mitochondria average670 µM matrix [Mg²⁺], a value that would permit <1%of maximumK⁺/H⁺antiport activity. Hypotonic swelling results in large decreases inmatrix [Mg²⁺], butswelling due to accumulation of acetate salts does not alter[Mg²⁺]. Swelling inphosphate salts decreases matrix[Mg²⁺], but not tolevels that permit appreciable antiport activity. We conclude that1) it is unlikely that matrix[Mg²⁺] serves as themitochondrial volume sensor, 2) ifK⁺/H⁺antiport functions as a volume control transporter, it is probably regulated by factors other than[Mg²⁺], and3) alternative mechanisms formitochondrial volume control should be considered.

     

The participation of phosphate in the formation of a carrier for the transport of Mg++ and Mn++ ions into yeast cells

During the absorption of phosphate by yeast, the cells acquire the capacity to absorb Mn⁺⁺ and Mg⁺⁺, a capacity which is retained even after phosphate is no longer present in the medium. Cells pretreated with phosphate and then washed, slowly lose their ability to absorb Mn⁺⁺, the rate of loss depending on the temperature and on the metabolic state. The fermentation of sugars induces a very rapid loss of absorptive capacity, whereas the respiration of ethyl alcohol, lactate, or pyruvate has little effect. Inhibitor studies with sodium acetate, redox dyes, and arsenate, reveal parallel effects on Mn⁺⁺ absorption, and on phosphate absorption. It is concluded that the synthesis of a carrier for the transport of Mg⁺⁺ and Mn⁺⁺ involves a phosphorylation step closely coupled with reactions involved in the absorption of phosphate.     

Aluminium induces rapid changes in cytosolic pH and free calcium and potassium concentrations in root protoplasts of wheat (Triticum aestivum)

Addition of aluminium chloride (50 μM Al) caused different effects on the transmembrane electrical potential (PD) of root cells in Al-tolerant wheat (Triticum aestivum) cv. Kadett and Al-sensitive cv. WW 20299. As changes in PD of plant cells may depend on transient fluxes of protons, potassium and/or calcium through cell membranes, the effect of Al was investigated on the cytosolic concentrations of these ions in protoplasts isolated from root tips of the same cultivars. The tetra[acetoxymethyl] esters of the fluorescent dyes bis-carboxyethyl-carboxyfluorescein, BCECF, K⁺-binding benzofuran isophthalate, PBFI, and the stilbene chromophore Fura 2-AM were used to determine pH, K⁺ and Ca²⁺, respectively. Changes in fluorescence ratios, directly reflecting changes in [H⁺], [K⁺] and [Ca²⁺] in the cytosol, were determined by photometry fluorescence microscopy. Additions and removals of Al to and from both cultivars caused hyperpolarizations and depolarizations, respectively, but only in the sensitive cv. WW 20299 did the resting PD decrease gradually. Addition of Al to the protoplasts caused rapid changes in cytosolic pH, free [K⁺] and [Ca²⁺]. In both cultivars Al caused a transient oscillating increase in cytosolic [Ca²⁺] for 1 or 2 min and a rapid pH-dependent change in cytosolic [K⁺]. At pH 5 the presence of K⁺ in the medium diminished the Al-induced decrease in cytosolic [K⁺]. Aluminium (50 μM) induced a transient increase in cytosolic [H⁺] (pH decreased) in both cultivars, but the cytosolic pH returned to its initial value only in the Al-tolerant cv. Kadett. In the Alsensitive cv. WW 20299, repeated additions of Al caused a gradual decline in pH. Moreover, in the presence of 1 mM KCl, pH recovered completely in both cultivars. Since only the effect on pH differed in the two cultivars, the more toxic effect of Al on the cv. WW 20299 should be related to the change in pH.     

Regional high affinity synaptosomal transport of choline in mouse brain — Influence of oxotremorine treatment

Kinetic parameters for high affinity [HA] uptake $\text{in vitro}$ in synaptosomes from different mouse brain regions were investigated. V_max was highest in the striatum [200 pmol.· mg protein^?1 · 4 min^?1], followed by the cortex [111 pmol · mg protein^?1 · 4 min^?1], hippocampus [63 pmol · mg protein^?1 · 4 min^?1], midbrain [21 pmol · mg protein^?1 · 4 min^?1] and, lowest, medulla oblongata [5 pmol · mg protein^?1 · 4 min^?1]. K_m was about the same in all brain regions [0.9–1.4 μM]. No sign of HA uptake was detected in synaptosomes from the cerebellum. A clear relationship between V_max for synaptosomal HA uptake of Ch $\text{in vitro}$ and apparent turnover of ACh $\text{in vivo}$ was found between the brain regions. Administration of oxotremorine [1 mg·kg^?1 i.p.] decreased V_max for HA uptake of Ch by 60% in the cortex and hippocampus, by 50% in the striatum and by 20% in the midbrain. This effect is in accordance with the previously observed marked decrease in turnover of ACh in these brain regions following oxotremorine treatment.     

Na+ and H+ dependent Mn2+ binding to phosphatidylserine vesicles as a test of the Gouy-Chapman-Stern theory

Summary Mn²⁺ binding to phosphatidylserine (PS) vesicles was measured by EPR as a function of [Na⁺] and pH. At nearly physiological monovalent salt concentration the apparent Mn²⁺ affinity (K _a) increased monitonically over the pH range 5.7–8.35, withK _a roughly [H⁺]^–1 above pH 7.3. It was found, moreover, thatK _a fell off more rapidly with added NaCl at pH 6.1 than at pH 7.87. Qualitatively, these results are consistent with two types of Mn²⁺-PS binding: (i) simple adsorption and (ii) adsorption with the release of an amino proton from PS. The existence of Mn²⁺-induced H⁺ displacement from PS was verified through titration measurements, employing a pH electrode.When H⁺ displacement is taken into account, the variation inK _a with [Na⁺] observed at pH 6.1 is found to be in reasonably good agreement with that expected from the Gouy-Chapman-Stern theory of ionic binding to charged surfaces.     

Calcium regulation of skeletal myogenesis. I. Cell content critical to myotube formation

Summary Primary cultures of embryonic chick pectoral skeletal muscle were used to study calcium regulation of myoblast fusion to form multinucleated myotubes. Using atomic absorption spectrometry to measure total cellular calcium and the⁴⁵Ca-exchange method to determine free cellular Ca⁺⁺, our data suggest that only the free cellular calcium changes significantly during development under conditions permissive for myotube formation (0.9 mM external Ca⁺⁺). Increases in calcium uptake occurred before and toward the end of the period of fusion with the amount approximating 2 to 4 pmol per cell in mass cultures. If the medium [Ca⁺⁺] is decreased to 0.04 mM, as determined with a calcium electrode, a fusion-block is produced and free cell Ca⁺⁺ decreased 5- to 10-fold. Removal of the fusion-block by increasing medium [Ca⁺⁺] results in a release of the fusion-block and an increase in cellular Ca⁺⁺ to approximately 1 pmol per cell during fusion, and higher thereafter. Cation ionophore A23187 produced transient increases in cellular calcium and stimulated myoblast fusion and the final extent of myotube formation only when added at the onset of culture. Results suggest that transient increased calcium uptake alone is insufficient for fusion because critical cellular content in conjunction with permissive amounts of medium [Ca⁺⁺] must exist. The latter suggests further that cell surface Ca⁺⁺ was also critical.     

Phosphoglycerate mutase in developing forespores of Bacillus megaterium may be regulated by the intrasporal level of free manganous ion.

When young intact forespores of Bacillus megaterium were incubated with either Mn⁺⁺ or the ionophore X-537A, the pool of 3-phosphoglyceric acid (3-PGA) was stable. However, incubation of forespores with Mn⁺⁺ plus the ionophore X-537A resulted in rapid and complete utilization of the 3-PGA. This effect was not seen with Ca⁺⁺ or Mg⁺⁺, and was also not observed with older forespores or fresh dormant spores. Since the phosphoglycerate mutase of $\text{B.}\text{megaterium}$ has an absolute and specific requirement for Mn⁺⁺, it is possible that phosphoglycerate mutase in developing forespores may be inactive because of a low intrasporal level of free Mn⁺⁺.     

Requirements of Hsp104p activity and Sis1p binding for propagation of the [RNQ+] prion

The formation and maintenance of prions in the yeast Saccharomyces cerevisiae is highly regulated by the cellular chaperone machinery. The most important player in this regulation is Hsp104p, which is required for the maintenance of all known prions. The requirements for other chaperones, such as members of the Hsp40 or Hsp70 families, vary with each individual prion. [RNQ⁺] cells do not have a phenotype that is amenable to genetic screens to identify cellular factors important in prion propagation. Therefore, we used a chimeric construct that reports the [RNQ⁺] status of cells to perform a screen for mutants that are unable to maintain [RNQ⁺]. We found eight separate mutations in Hsp104p that caused [RNQ⁺] cells to become [rnq⁻]. These mutations also caused the loss of the [PSI⁺] prion. The expression of one of these mutants, Hsp104p-E190K, showed differential loss of the [RNQ⁺] and [PSI⁺] prions in the presence of wild type Hsp104p. Hsp104p-E190K inefficiently propagated [RNQ⁺] and was unable to maintain [PSI⁺]. The mutant was unable to act on other in vivo substrates, as strains carrying it were not thermotolerant. Purified recombinant Hsp104p-E190K showed a reduced level of ATP hydrolysis as compared to wild type protein. This is likely the cause of both prion loss and lack of in vivo function. Furthermore, it suggests that [RNQ⁺] requires less Hsp104p activity to maintain transmissible protein aggregates than Sup35p. Additionally, we show that the L94A mutation in Rnq1p, which reduces its interaction with Sis1p, prevents Rnq1p from maintaining a prion and inducing [PSI⁺].Key words: [RNQ⁺], [PSI⁺], Hsp104p, Sis1p, mutagenesis     

Nuclear suppressors of the [poky] cytoplasmic mutant in Neurospora crassa. III. Effects on other cytoplasmic mutants and on mitochondrial ribosome assembly in [poky].

Summary We have previously isolated six non-allelic, nuclear mutations (su ^I loci) that partially suppress the growth, respiratory and cytochrome abnormalities of the extranuclear [poky] mutant.A comparison of the mitochondrial ribosome profiles of suppressed and unsuppressed [poky] strains revealed that five of the six suppressors alleviate at least partially the deficiency of mitochondrial small ribosomal subunits that is associated with the [poky] genotype.Six independently isolated Group I extranuclear mutants, namely [exn-1], [exn-2], [exn-4], [stp-B ₁], [SG-1] and [SG-3], which have growth and cytochrome phenotypes similar to [poky], also were found to be deficient in small subunits of mitochondrial ribosomes. Using cytochrome aa ₃ and b production as a criterion for mitochondrial protein synthesis, it could be shown that the nuclear su ^I suppressors of [poky] also suppress the other six Group I extranuclear mutants. However, differences in the efficiencies of suppression by su ^I suppressors suggest that at least some of Group I extrachromosomal mutants are not simply re-isolates of [poky], but represent distinct extranuclear mutations.     

Electrical properties of Paramecium caudatum: all-or-none electrogenesis

Summary Specimens of Paramecium immersed in solutions of CaCl₂ show graded electrogenesis in response to imposed transmembrane current. However, when BaCl₂ in a final concentration of 0.25 mM is added to a 1 mM CaCl₂ solution, an outward current pulse of 10^-10 amp or greater elicits an all-or-none transient reversal in membrane potential having a duration of about 40 msec. An increase of [Ba⁺⁺] results in (a) lower resting potential, (b) positive shift in critical firing level, (c) increased overshoot of the action potential, (d) decreased hyperpolarizing afterpotential, and (e) increased duration of the action potential (a.p.). If [Ca⁺⁺] is increased along with [Ba⁺⁺] so as to keep the ratio [Ba⁺⁺]/[Ca⁺⁺] constant, the same results are obtained except that the duration of the a. p. remains unaltered. Thus, effects a-d appear to be related to [Ba⁺⁺] and not to [Ca⁺⁺] or [Cl^-]. The degree of overshoot in 1 mM Ca is linearly related to log [Ba⁺⁺] with a slope of approximately 22 mv. With the ratio [Ba⁺⁺]/[Ca⁺⁺] constant, the slope closely approaches the ideal value of 29 mv. The evidence indicates that prolongation of the action potential is due to a delayed onset of Ba inactivation, and that this in turn is a function of surface-bound Ba. Other features of the action potential are absolute refractoriness during its rising and plateau phases, relative refractoriness lasting several seconds, and repetitive firing in response to steady current depolarization. The response is unaffected by TTX and TEA. Mn prolongs the action potential. Sr has an action similar to Ba, whereas the addition of K, Na, Rb, or Mg to the basic calcium medium is unaccompanied by all-or-none electrogenesis.On leave of absence from the Zoological Institute, Faculty of Science, University of Tokyo.Support came from National Science Foundation grant GB-5752x, U.S.P.H.S. grant NB-03664, and in part from Office of Naval Research grant Nonr 4785(00) administered by the Marine Biological Laboratory, Woods Hole.