Circular dichroism and saccharide-induced conformational transitions of lectins from Ricinus communis.

Conformational studies on lectins from castor beans (Ricinus communis), RCA_I and RCA_II, were performed by using circular dichroism (CD). The CD spectra were similar showing several negative bands at 270–320 nm, a positive region at 230–250 nm, several negative bands at 205–225 nm, and a positive peak at about 195 nm. However, significant differences were observed in the band strength between RCA_I and RCA_II. Lactose, melibiose, and d-fucose induced marked Conformational alterations in RCA_I, whereas weaker effects were produced by d-galactose and l-rhamnose. Saccharide-induced conformational alterations were weaker in RCA_II than in RCA_I, with only lactose and melibiose inducing significant alterations. d-Glucose and 2-acetamido-2-deoxy-d-glucose, which do not inhibit hemagglutination by RCA_I or RCA_II, did not influence lectin conformation. Acetylation of tyrosyl groups with N-acetylimidazole produced changes in the CD bands in the near uv indicating involvement of tyrosine residues. The saccharide effect was most pronounced at 285 nm, a band that was assigned to a tyrosine chromophore. Analysis of the CD bands in the far-uv zone indicated the presence of approximately 50% pleated sheet (β) structure, and 13–15% α-helix in both RCA_I and RCA_II. According to the CD results, the polypeptide chain backbone in the lectins was not affected by the saccharides, whereas significant disorganization occurred in 7 m guanidine-HCl.     

Conformational features of bradykinin. A circular dichroism study of some peptide fragments and structural analogues of bradykinin.

The vasoactive hormone bradykinin, its N-and C-terminal fragments and some structural analogues were studied by Circular Dichroism. Conformational features of the peptide can be detected by comparative analysis of the various CD spectra recorded as a function of aqueous pH, solvent and temperature. It is shown that the two biologically essential arginine residues (Arg1 and Arg9) are important for the specific folded bradykinin conformation. Differences between bradykinin, its fragments and analogues become clearly established in conformational terms, and are discussed in relation to the biological activity of these peptides.     

All three chains of 1 alpha 2 alpha 3 alpha collagen from hyaline cartilage resist human collagenase

A previous report that the 3 alpha collagen chain of hyaline cartilage was cleaved by human collagenase could not be confirmed when the 1 alpha 2 alpha 3 alpha collagen fraction was freed of all contaminating type II collagen. All three minor collagen chains, 1 alpha, 2 alpha and 3 alpha, were totally resistant to highly purified collagenases from both rheumatoid synovial and gastric mucosal tissues. This finding and CNBr-peptide patterns suggest that, despite the close homology with alpha 1 (II), the 3 alpha chain is a unique collagen component, possibly combined with 1 alpha and 2 alpha in heterotrimeric molecules. In contrast, a 3 alpha-like component from fibrocartilage was cleaved by collagenase and gave a CNBr-peptide pattern more typical of alpha 1 (II) than of the collagenase-resistant 3 alpha of hyaline cartilage.     

The preparation and study of some novel glycosides of D-galactose

The tert-butyl- and the 2,2,2-trichloroethyl α- and β-D-galactopyranosides were prepared and both α-D-glycosides were selectively benzoylated to give the 2,3,6-tri-O-benzoyl-D-galactopyranosides. Cleaving of the glycosidic groups is described. The glycosides are useful intermediates for oligosaccharide synthesis where generation of a reducing sugar terminus under mild conditions is necessary.     

Insulin polymorphism: some physical and biological properties of rat insulins

Although rat insulins I and II show no significant differences in their biological activities and receptor binding on isolated fat cells, X-ray studies and circular dichroism indicate that they have differences in their structures. Rat insulin II forms zinc insulin hexamers in an identical manner to bovine insulin, but insulin I, which has a unique proline substitution at B9, forms hexamers less easily. Rat insulin I can form zinc insulin hexamers given higher zinc concentrations, as indicated by the formation of rhombohedral 2Zn insulin crystals. On the other hand, rat insulin II forms cubic crystals of space group $\text{P4}{}_2\text{32}\text{with}\text{a = 67}\text{A}\text{?}$ under similar conditions. Model building indicates that these crystals contain a tetrahedral arrangement of zinc hexamers. They have a higher solvent content and are less stable than rhombohedral insulin crystals. The relation of these observations to the rat insulin storage granules and the importance of polymorphism to the physiology and evolution of insulin are discussed.     

Thyrotropin-releasing hormone and a homologous peptide in the reproductive system of the female rat and pig

TRH and a TRH homologous peptide have been shown to occur throughout the female rat and pig reproductive systems by TRH radioimmunoassay, SP-Sephadex C-25 cation exchange chromatography, and parallel line analysis of the assays. The total amount of TRH and TRH homologous peptide immunoreactivity was highest in the oviducts followed by the ovary and then uterus. The concentration of TRH immunoreactivity in all reproductive organs of the rat fell gradually from one month of age. TRH and the TRH homologous peptide were not parallel on serial dilution and measurement in the same TRH radioimmunoassay. The rapid degradation of TRH by pig follicular fluid may explain the higher measured concentration of TRH homologous peptide compared to TRH not only in pig follicular fluid but also in the pig ovary as a whole.     

Quantitative determination of amino acid racemization in heat-alkali-treated melanotropins: Implications for peptide hormone structure-function studies

The treatment of frog skins (in vitro) and frogs (in vivo) with melanotropins that have been heated briefly in aqueous alkali resulted in prolonged skin darkening. It has been postulated that this increase in melanotropic activity is related to the partial racemization of amino acid residues of the melanotropins. Quantitative determination of the extent of racemization of eight amino acids (Val, Pro, Met, Phe, Glu, Asp, Nle, Ser) present in α-melanotropin (α-MSH), [4-norleucine]-α-MSH, β_porcine-melanotropin (β_p-MSH), and [7-norleucine]-β_p-MSH after brief heat-alkali treatment, was accomplished using a high-resolution gas chromatographic technique. Phenylalanine-7 in α-MSH and [4-norleucine]-α-MSH and phenylalanine-10 in β_p-MSH and [7-norleucine]-β_p-MSH were found to be partially racemized to a greater extent than expected. Other amino acid residues were also racemized to unexpected degrees. The subsequent synthesis of an α-MSH analog containing d-phenylalanine-7, [4-norleucine, 7-d-phenylalanine]-α-MSH, resulted in a highly potent melanotropin with ultralong biological activity, as determined by frog skin bioassay, stimulation of mouse melanoma cell tyrosinase activity, and activation of mouse melanoma adenylate cyclase.     

Synthesis and biological properties of 9-deoxo-16,16-dimethyl-9-methylene-PGE2

The in vivo monkey uterine stimulating potency of 9-deoxo-16,16-dimethyl-9-methylene-PGE₂ is similar to that of 16,16-dimethyl-PGE₂ and approximately 15 times that of PGE₂. Low doses of this compound stimulated uterine contractions when administered vaginally. Pregnancy was terminated prematurely following subcutaneous, intramuscular or vaginal suppository treatment. Estimates of potential for gastrointestinal side effects using the rat enteropooling assay and in vivo monkey effects indicate that diarrhea will be substantially reduced with retention of uterine stimulating potency.     

Studies on the generation of hydrogen peroxide during some non-enzymic reactions changing the hyaluronic acid molecule

The effect of catalase on non-enzymic-induced changes in the conformation of hyaluronic acid in a vitreous humour preparation was measured using viscometry. Ascorbate, heavy metal ions, riboflavin or EDTA all lowered the viscosity of hyaluronic acid solutions. These effects could be prevented by the addition of catalase. This suggested that H₂O₂ is produced by these compounds and that the resulting change in conformation of hyaluronic acid may be due to peroxyl and hydroxyl attack by the free radicals thus generated.     

Depletion of intracellular putrescine and spermidine by alpha-difluromethylornithine does not inhibit proliferation of 9L rat brain tumor cells.

Incubation of 9L rat brain tumor cells with 25 mM DL-α-difluoromethylornithine inhibits cell proliferation, while treatment with 10 mM and 1 mM do not. All three concentrations cause equal degrees of depletion of intracellular putrescine and spermidine content, but have no effect on spermine content. These observations show that 9L cells can continue to proliferate in spite of significant polyamine depletion and leads one to question the role of polyamines in 9L cell replication. These observations also suggest that inhibition of 9L cell proliferation by 25 mM DL-α-difluormethylornithine is probably not due to its effect on ornithine decarboxylase or on intracellular polyamine content.     

Subcellular localization and some properties of the adenylate cyclase activity of the yeast, Saccharomyces cerevisiae

Saccharomyces cerevisiae was grown in the presence of 5% (w.v) Glucose and converter to protoplasts. The total particulate material obtained from lysed protoplasts was fractionated by sucrose density gradient ultracentrifugation and the distribution of adenylate cyclase throughout the gradient determined. Adenylate cyclase activity was found to be larger associated whith intracellular particulate fractions. Little activity was found in the plasma membrane-rich fraction.The adenylate cyclase activity was found to be inhibited by F^?, pyrophosphate and aminophylline, whereas glucagon, 5-hydroxytryptamine and concanavalin A were without effect.The enzymic activity appeared to be modulated by “catabolite repressors” (glucose, fructose and α-methylglucoside) as well as by acetate. A possible role for adenylate cyclase in regulating the levels of cyclic AMP in the cell during glucose repression is suggested.     

Circular dichroism and the conformational properties of soybean beta-amylase

The conformational properties of soybean β-amylase were investigated by the circular dichroism probe and measurement of enzyme activity. The enzyme exhibited a positive circular dichroism band at 192 nm, a negative band at 222 nm, and a shoulder near 210 nm. Analysis of the spectrum in the far ultraviolet zone indicated the presence of approximately 30% of α helix and 5–10% of β-pleated sheet, the rest of the polypeptide main chain possessing aperiodic structure. In the near ultraviolet reagion, the enzyme protein showed at least six positive peaks at 259, 265, 273, 281, 292, and 297 nm. The positive bands at 292 and 297 nm remained unaltered on acetylation of the enzyme by N-acetylimidazole and were assigned to tryptophanyl chromophores. These bands were affected in intensity in the presence of maltose or cycloheptaamylose, which indicates that some tryptophan residues are situated at the binding sites. The native conformation of soybean β-amylase was found to be sensitive to pH variation (below pH 5 and above pH 10), sodium dodecyl sulfate, guanidine hydrochloride, and heating to 50–55 °C. Complete disorganization of the secondary structure was attained by 6 m guanidine hydrochloride. Sodium dodecyl sulfate was effective in disturbing the tertiary structure of the enzyme but did not affect significantly the secondary structure. Enzymatic inactivation was paralleled by the decrease of circular dichroism bands in the near ultraviolet region as produced by the denaturants. It is concluded that the uniquely folded structure of the enzyme contains some less rigid domains and a rigid core stabilized by hydrophobic interactions, electrostatic interactions, and hydrogen bonds.     

The reaction between N-ethylmaleimide and ribosomes. A re-examination of some common assumptions.

The rates of the reaction between N-ethylmaleimide and protein sulfhydryl groups vary considerably from protein to protein, and are slower than the model reaction with cysteine. Thus, the assumption that N-ethylmaleimide alkylates ribosomal protein sulfhydryl groups very rapidly, an assumption which has been made in certain discussions of ribosomal protein structure, is a doubtful one.     

Cerebral endothelial cell culture. I. The presence of beta 2 and alpha 2-adrenergic receptors linked to adenylate cyclase activity

Cultured endothelial cells derived from cerebral microvessels separated from 2-day-old rat brain contain a specific beta 2 and alpha 2-adrenergic sensitive adenylate cyclase (AC). Among the various tested hormones, PGE1 and PGE2 were found to be the most potent activators, while adenosine, angiotensin I and II, gamma-aminobutyric acid and vasoactive intestinal peptide inhibited the enzyme activity. However, acetylcholine, histamine, serotonin, glycine, glutamine, bradykinin, neurotensin and vasopressin (Lysine and Arginine) had no effect on the adenylate cyclase activity in this model. The susceptibility of the cerebrovascular endothelial AC system to the vasoactive substances as well as presence of beta 2 and alpha 2-type adrenergic receptors in the cultured endothelium provides additional support for the proposed endothelial involvement in the regulation of cerebrovascular permeability and blood flow.     

Synthesis of tetrazoles from some per-O-acetylaldononitriles

Synthesis of 5-(polyacetoxyalkyl)tetrazoles from some acetylated aldononitriles by reaction with ammonium azide is described. Deacetylation of these compounds afforded the corresponding 5-(polyhydroxyalkyl)tetrazoles.     

Further facile immobilization of enzymes on hydrous metal oxides and use of their immobilization reversibility phenomena for the recovery of peptide antibiotics

Practical aspects of the facile immobilization of enzymes on hydrous metal oxides, a well-established means of enzyme-movement restriction, are described. Various enzymes (e.g. glucoamylase, peroxidase, dextranase) have been immobilized by chelation of several hydrous metal oxides, those of titanium(IV) and zirconium(IV) proving to be the most satisfactory for practical purposes. Localization of the gel into a granular form could be achieved successfully with good enzyme-immobilization characteristics by using ion-exchange resin as an internal matrix. The immobilization process was highly efficient for the relative proportions of hydrous oxide to enzyme used, with usually >90% of the available protein being insolubilized. Retention of enzyme activity was generally very good and was stable to reuse and to conventional buffer conditions. Activities of the immobilized enzymes were partially stable to lyophilization or drying of the hydrous oxide gels. Modification of the hydrous metal oxide surface by drying or treatment with phosphate or carbonate led to a decrease in complexing ability. The effect of carbonate can be circumvented by lowering the pH of the solution to around 5 and removing any carbon dioxide formed, by aeration. Such treatment allowed compounds to chelate to hydrous zirconium oxide(IV) in the presence of carbonate and therefore the hydrous oxide could be applied successfully to the concentration of peptide antibiotics from the fermentation medium in which they are being produced, including production at low concentrations.     

Mutagenesis and anti-mutagenesis in Salmonella: influence of ethionine and caffeine on yields of mutations induced by 2-aminopurine and 9-aminoacridine

Ethionine, the ethyl analogue of methionine, slightly reduced the yield of reversions of the hisC3076 frameshift marker induced by 9-aminoacridine (9AA) in an excision-proficient strain of Salmonella typhimurium, but completely abolished mutagenesis genesis by 9AA in the excision-deficient uvrB-deletion strain TA1537. No toxic effects of ethionine were apparent in either the excision-proficient or the excision-deficient strain. Because of the differential effects of ethionine on mutagenesis in the two strains, it seemed possible that an ethionine-sensitive step in the process(es) leading to fixation of 9AA-induced mutations might be compensated for by the uvrA,B,C⁺ excision-repair system. To further test this possibility, we used caffeine (a compound known to significantly reduce the efficacy of the excision-repair process) as a co-treatment with ethionine for cells of an excision-proficient strain exposed to 9AA. Treatment with caffeine alone or ethionine alone had very little effect on reversion yield, whereas co-treatment with the two agents abolished 9AA mutagenesis. It appeared, therefore, that either the caffeine-sensitive pathway or the ethionine-sensitive pathway needed to be functioning if 9AA-induced reversions of the hisC3076 marker were to be detected. Addition of methionine to cells of the excision-deficient strain exposed to 9AA restored their ability to be mutated by 9AA, however. In a base-pair substitution back-mutation system, ethionine slightly enhanced the yields of revertants of the trpE8 marker induced by 2-aminopurine (2AP) in both an excision-proficient strain (at all 2AP dose levels tested) and an excision-deficient strain (only at the lower dose levels). In the excision-deficient strain, doses of 2AP above 300 μg/plate were highly toxic when ethionine was also present. It was for this reason that no 2AP-induced revertants were recovered at the higher 2AP concentrations. Treatment of the trpE8 strain with methionine also enhanced the yield of 2AP-induced revertants of this marker.