Interaction of cytochrome c with lipid monolayers

Cytochrome c was permitted to react with several lipid monolayers in which surface pressure, lipid charge and unsaturation were varied. Cytochrome c interaction with the films caused increased surface pressures, and the magnitude and rate of surface pressure change were compared under a variety of experimental conditions. Large surface pressure changes were associated with more expanded films, whereas greater rates of surface pressure change were associated with favorable charge interaction between cytochrome c and the films. Under the most favorable conditions, rates of surface pressure change were limited principally by protein diffusion to the interface. From these data, it is suggested that unsaturation in lipids of biological membranes may help stabilise non-polar protein-lipid interactions, whereas charge interaction may facilitate and direct initial binding of protein to membranes.     

The effect of oxygen on 14CO2 fixation in mesophyll cells isolated from Digitaria sanguinalis (L.) Scop. leaves

Mesophyll cells were isolated from fully-expanded leaves of $\text{Digitaria sanguinalis}$ (L.) Scop. by a combined maceration-filtration technique. In the presence of pyruvate, photosynthetic ¹⁴CO₂ uptake in the isolated cells was not inhibited by atomospheric levels of oxygen. In contrast, superatmospheric levels of oxygen substantially inhibited the light-dependent fixation of ¹⁴CO₂. These oxygen effects are similar to those observed with intact C4 leaves and suggest that the lack of inhibition of C4 photosynthesis by atmospheric levels of oxygen results from the relative oxygen-insensitivity of the phosphopyruvate carboxylase-CO₂ pump in the mesophyll.     

Lipophilicity and catalysis of photophosphorylation. II. Quinoid compounds as artificial carriers in cyclic photophosphorylation and photoreductions by Photosystem I

The topography of the chloroplast membrane has been studied using the following pairs of quinoid compounds with similar structure and chemical properties, but with different lipid solubility: phenazine/sulfophenazine, naphthoquinone/naphthoquinone sulfonate, indophenol/sulfoindophenol and lumiflavin/FMN.

All these compounds in the oxidized form are able to accept electrons from the photosynthetic electron transport chain in Hill reactions. However, only the lipophilic compounds in the reduced form can donate electrons to Photosystem I, when electron flow from Photosystem II is blocked by inhibitors. This is in agreement with the notation that the oxidizing site of Photosystem I (P₇₀₀⁺) and the electron donors for Photosystem I (cytochrome f and plastocyanin) are located inside the lipid barrier of the inner chloroplast membrane. The reducing sites in the Hill reactions must be located on the outer surface, accessible from the suspending medium.

It has been known for a long time that N,N′-tetramethyl-p-phenylenediamine can donate electrons to Photosystem I, but contrary to diaminodurene (2,3,5,6-tetramethyl phenylenediamine) it does not induce ATP formation. Both compounds are lipophilic and have similar redox potentials, but only the latter carries hydrogens which are involved in the redox reaction. For energy conservation, coupled to electon flow in Photosystem I, it therefore seems necessary that the lipophilic redox compound in the reduced form can carry hydrogens through the chloroplast membrane.     

Requirement of galactolipids for Photosystem I activity in lyophilized spinach chloroplasts

1. The effect of monogalactosyl diacylglycerol and digalactosyl diacylglycerol on reconstitution of Photosystem I activity in heptane-extracted and galactolipase-treated spinach chloroplasts was investigated.2. Both galactolipids, in a molar ratio with chlorophyll of 2.5, partially restored Photosystem I activity in heptane-extracted chloroplasts. An addition o saturating amounts of plastocyanin caused complete reactivation of Photosystem I.3. Similarly, with galactolipase-treated chloroplasts, both galactolipids partially restored Photosystem I activity and additional amounts of plastocyanin were required for complete reactivation.4. The action of galactolipids on partial reconstitution of Photosystem I supports the suggestion of their structural role in the restoration of thylakoid membranes.     

Detection of sequences with Z-DNA forming potential in higher plants

Sequences of alternating purine-pyrimidine residues with Z-DNA forming potential have been detected in the nuclear DNA of two higher plant species: wheat and radish. Poly (dG-dT) and poly (dG-dC) stretches have been detected by hybridization of the corresponding nick-translated probes to Southern blots. These stretches are scattered throughout the genome and some of them belong to moderately repeated sequence families interspersed with other DNA sequences.     

Differentiation between mutants of Escherichia coli K12 defective in oxidative phosphorylation

Hybrid membrane particles from two mutants of Escherichia coli K₁₂, B_v4 and K_I1, defective in oxidative phosphorylation, have been prepared, in which ATP-driven membrane energization is restored.

A soluble factor of mutant K_I1 was found to have properties similar to parental crude coupling factor, ATPase (EC 3.6.1.3). Membrane particles of this mutant could not be reconstituted by parental coupling factor. Either parental coupling factor, or the soluble factor of mutant K_I1 could reconstitute both respiration-driven and ATP-driven energization to membrane particles of mutant B_V4 or to parental particles depleted of ATPase. Mutant B_V4 was found to be devoid of coupling factor activity, while retaining the ability to hydrolyze ATP. Both mutants possess an ATPase with an altered binding to the membrane.

Mutant K_I1 is impaired in respiration-driven amino acid transport, in contrast to mutant B_V4.

The three major subunits of parental Escherichia coli ATPase have been isolated and antibodies have been prepared against these subunits. Antibodies against the largestsubunit ( component) or against the intact catalytic subunits ( + β components) inhibit both ATP-P_i exchange in the parent organism as well as ATP hydrolytic activity in parent and mutants. Antibodies against the two other subunits (β or γ components) also inhibit these two reactions, but were found to be less effective. Mutant N_I44, which lacks ATPase activity, shows no precipitin lines with anti-, anti-β, anti-γ, or anti-( + β) preparations. In contrast, mutants B_V4 and K_I1, exhibit cross-reactivity with all of the antisera.     

Tonofilament protein, a keratin from rat epidermis

Tonofilament protein from newborn rat epidermis was found to be antigenically related to mouse keratins. Tonofilament protein, like keratins, could be extracted with 8 M urea in Tris buffer. The yield was enhanced by the presence of dithiothreitol. A higher molecular weight (64,000 dalton) protein antigenically cross-reacting with tonofilament protein but with a slightly different amino acid composition was also extracted.     

Protein-SV40 DNA complex stable in high salt and sodium dodecyl sulfate.

A protein-DNA complex which is stable in concentrated salt solutions and in the presence of sodium dodecyl sulfate has been extracted from purified viruses and is found in the nicked circular DNA fraction. The protein is visualized as a “dot” on the DNA molecule by electron microscopy using a modified version of the ethidium bromide mounting technique. The position of the dot is at 0.67 genome units clockwise from the ecoRI restriction site on the SV40 DNA map.     

Flash-induced absorption changes of the primary donor of photosystem II at 820 nm in chloroplasts inhibited by low pH or tris-treatment

A comparative study is made, at 15 °C, of flash-induced absorption changes around 820 nm (attributed to the primary donors of Photosystems I and II) and 705 nm (Photosystem I only), in normal chloroplasts and in chloroplasts where O₂ evolution was inhibited by low pH or by Tris-treatment.At pH 7.5, with untreated chloroplasts, the absorption changes around 820 nm are shown to be due to P-700 alone. Any contribution of the primary donor of Photosystem II should be in times shorter than 60 μs.When chloroplasts are inhibited at the donor side of Photosystem II by low pH, an additional absorption change at 820 nm appears with an amplitude which, at pH 4.0, is slightly higher than the signal due to oxidized P-700. This additional signal is attributed to the primary donor of Photosystem II. It decays ($\text{t}{}_{\mathrm{<mtext>1</mtext><mtext>2</mtext>}}$ about 180 μs) mainly by back reaction with the primary acceptor and partly by reduction by another electron donor. Acid-washed chloroplasts resuspended at pH 7.5 still present the signal due to Photosystem II ($\text{t}{}_{\mathrm{<mtext>1</mtext><mtext>2</mtext>}}$ about 120 μs). This shows that the acid inhibition of the first secondary donor of Photosystem II is irreversible.In Tris-treated chloroplasts, absorption changes at 820 nm due to the primary donor of Photosystem II are also observed, but to a lesser extent and only after some charge accumulation at the donor side. They decay with a half-time of 120 μs.     

Conformational changes in coupling factor 1 may control the rate of electron flow in spinach chloroplasts.

The relationship between the rate of electron flow, internal H⁺ concentration and the magnitude of the H⁺ concentration gradient (ΔpH) in chloroplasts illuminated at various light intensities has been examined. At an external pH of 7.0, the internal H⁺ concentration is a linear function of the rate of electron flow except at saturating light intensity. In contrast, at pH 8.1, this relationship between electron flow and internal H⁺ concentration holds only at values of ΔpH below about 2.8 – 2.9 units. At higher ΔpH values, the rate of electron flow increases much more dramatically than the internal H⁺ concentration. ATP (0.1 mM) prevents this increase. It is suggested that at pH 8.1 but not at pH 7.0, the conformation of coupling factor 1 is altered at high ΔpH values. Its altered conformation may result in an increased efflux of H⁺ from the chloroplasts. This notion is supported by the effects of ATP on electron flow and ΔpH as well as the effect of external pH and light intensity on the reactivity of coupling factor 1 to N-ethylmaleimide.     

Identification of an artificial peptide motif that binds and stabilizes reduced human DJ-1

Although the precise biochemical function of DJ-1 remains unclear, it has been found to exert cytoprotective activity against oxidative stress. Cys106 is central to this function since it has a distinctly low pK_a rendering it extremely susceptible for oxidation. This characteristic, however, also poses a severe hindrance to obtain reduced DJ-1 for in vitro investigation. We have developed an approach to produce recombinant human DJ-1 in its reduced form as a bona fide basis for exploring the redox capacities of the protein. We solved the crystal structure of this DJ-1 at 1.56 Å resolution, allowing us to capture Cys106 in the reduced state for the first time. The dimeric structure reveals one molecule of DJ-1 in its reduced state while the other exhibits the characteristics of a mono-oxygenated cysteine. Comparison with previous structures indicates the absence of redox dependent global conformational changes in DJ-1. The capture of reduced Cys106 is facilitated by stabilization within the putative active site achieved through a glutamate side chain. This side chain is provided by a crystallographic neighbor as part of a ‘Leu–Glu’ motif, which was added to the C-terminus of DJ-1. In the structure this motif binds DJ-1 in close proximity to Cys106 through extended hydrophilic and hydrophobic interactions depicting a distinct binding pocket, which can serve as a basis for compound development targeting DJ-1.