Secondary transport of amino acids by membrane vesicles derived from lactic acid bacteria

Lactococci are fastidious bacteria which require an external source of amino acids and many other nutrients. These compounds have to pass the membrane. However, detailed analysis of transport processes in membrane vesicles has been hampered by the lack of a suitable protonmotive force (pmf)-generating system in these model systems. A membrane-fusion procedure has been developed by which pmf-generating systems can be functionally incorporated into the bacterial membrane. This improved model system has been used to analyze the properties of amino acid transport systems in lactococci. Detailed studies have been made of the specificity and kinetics of amino acid transport and also of the interaction of the transport systems with their lipid environment. The properties of a pmf-independent, arginine-catabolism specific transport system in lactococci will be discussed.Abbreviations pmf protonmotive force - transmembrane electrical potential - pH transmembrane pH gradient - PE phosphatidylethanolamine - PC phosphatidylcholine Paper adapted from a treatise Secondary Transport of Amino Acids by Membrane Vesicles Derived from Lactic Acid Bacteria and awarded the Kluyver Prize 1988 by the Netherlands Society of Microbiology.     

The molecular defect in propionic acidemia: Exon skipping caused by an 8-bp deletion from an intron in the PCCB allele

Propionic acidemia is an autosomal recessive metabolic disease resulting from a deficiency of propionyl CoA carboxylase (PCC) activity. To investigate the genetic basis of propionic acidemia, we isolated a cDNA encoding the precursor of the subunit of human PCC ( PCC). The cloned cDNA sequence was 1,832 bp long and the open reading frame of 1,617 nucleotides encoded a polypeptide of 539 amino acids with a molecular mass of 58,202 Da. The human PCC sequence shared a high degree of homology (91%) with the full-length cDNA of rat PCC at the amino acid level; there were only 47 differences among 539 amino acid residues compared. Polymerase chain reaction amplification and sequencing of cDNA from a subunit-deficient Japanese patient revealed a deletion of 101 nucleotides consisting of one exon from mature mRNA. This deletion resulted in a frameshift and a stop codon in the new frame. Analysis of the genomic DNA revealed a homozygous 8-bp deletion from bp3 to bp10 of the intron just downstream of the deleted exon. This deletion disrupted the consensus 5 splice signal and led to exon skipping.     

Production of thermostable amylolytic enzymes by Thermococcus hydrothermalis

A cell extract of Thermococcus hydrothermalis, grown for 6 h, gave -glucosidase activity at 14.9 U/l, degrading oligosaccharides and maltose. -Amylase, -glucosidase and pullulanase activities were detected at 289 U/l, 13.5 U/l and 30 U/l respectively in the culture medium after 24 h growth of the archaeum. All of three enzymes, characterised by a half-life time of 1 to 5 h at 95°C, degraded both the (14) and (16) linkages of polysaccharides and the (14) linkages of oligosaccharides. © Rapid Science Ltd. 1998     

C alpha and C beta carbon-13 chemical shifts in proteins from an empirical database

We have constructed an extensive database of 13C C and C chemical shifts in proteins of solution, for proteins of which a high-resolution crystal structure exists, and for which the crystal structure has been shown to be essentially identical to the solution structure. There is no systematic effect of temperature, reference compound, or pH on reported shifts, but there appear to be differences in reported shifts arising from referencing differences of up to 4.2 ppm. The major factor affecting chemical shifts is the backbone geometry, which causes differences of ca. 4 ppm between typical - helix and -sheet geometries for C, and of ca. 2 ppm for C. The side-chain dihedral angle 1 has an effect of up to 0.5 ppm on the C shift, particularly for amino acids with branched side-chains at C. Hydrogen bonding to main-chain atoms has an effect of up to 0.9 ppm, which depends on the main- chain conformation. The sequence of the protein and ring-current shifts from aromatic rings have an insignificant effect (except for residues following proline). There are significant differences between different amino acid types in the backbone geometry dependence; the amino acids can be grouped together into five different groups with different , shielding surfaces. The overall fit of individual residues to a single non-residue-specific surface, incorporating the effects of hydrogen bonding and 1 angle, is 0.96 ppm for both C and C. The results from this study are broadly similar to those from ab initio studies, but there are some differences which could merit further attention.     

The influence of nearest neighbors on the rate and pattern of spontaneous point mutations

Summary The numbers and local sequence environments of the two types of substitution mutation plus additions and deletions have been obtained directly in this study from differences between a large number of extant primate gene and pseudogene sequences. A total of 3786 mutations were scored in regions where similarities between pseudogene and corresponding gene sequences is 85%, comprising 30% of the pseudogene database of 80,584 bp. The pattern of mutations obtained in this fashion is almost identical to that obtained by Li et al. (1984) using a slightly different, more direct approach and with a smaller database. When mutations were scored, the neighbor pairs on the 5 and 3 sides were also noted, leading to a large 16 × 12 matrix of transitions and transversions. Biases of varying magnitude are found in the rates of substitution of the same base pair in different local sequence environments. The overall order for the effect of the 5 neighbor on the rates of substitution mutation of a pyrimidine is A > C T > G, and G > A > T > C for the 3 neighbor; where these results represent the average of substitution rates for the complement purine with complement neighbors of bases ordered above. The order for the 3 neighbor is essentially the same for the two transitions and most of the four transversions as well; however, the order for the 5 neighbor is more variable. The overall rate for the C · G T · A transition is not unusual, however the presence of a 3 neighboring G · C pair boosts the rate substantially, presumably due to specific cytosine methylation of the CG doublet in primate DNAs. The rate of the T · A C · G transition is also well above average when the 3 neighbor is an A · T, and to a lesser extent a G · C, pair. The latter bias is typical in that it reflects the association of alternating pyrimidine-purine sequences with increasing mutation rates. The substitution of the pyrimidine in a 5 purine-pyrimi-dine-purine3 sequence generally occurs much faster than in a pyrimidine tract and points to the local conformation as a major determining factor of the substitution rate. An apparent inverse relationship is found between starting and product doublet frequencies of base pairs undergoing mutations with specific 3 neighbors, indicating that differences in intrinsic substitution rates of base pairs with specific neighbors are a key factor in producing the familiar biases of nearest-neighbor frequencies.Offprint requests to: R. D. Blake     

Protein backbone angle restraints from searching a database for chemical shift and sequence homology

Chemical shifts of backbone atoms in proteins are exquisitely sensitive to local conformation, and homologous proteins show quite similar patterns of secondary chemical shifts. The inverse of this relation is used to search a database for triplets of adjacent residues with secondary chemical shifts and sequence similarity which provide the best match to the query triplet of interest. The database contains 13C, 13C, 13C, 1H and 15N chemical shifts for 20 proteins for which a high resolution X-ray structure is available. The computer program TALOS was developed to search this database for strings of residues with chemical shift and residue type homology. The relative importance of the weighting factors attached to the secondary chemical shifts of the five types of resonances relative to that of sequence similarity was optimized empirically. TALOS yields the 10 triplets which have the closest similarity in secondary chemical shift and amino acid sequence to those of the query sequence. If the central residues in these 10 triplets exhibit similar and backbone angles, their averages can reliably be used as angular restraints for the protein whose structure is being studied. Tests carried out for proteins of known structure indicate that the root-mean-square difference (rmsd) between the output of TALOS and the X-ray derived backbone angles is about 15°. Approximately 3% of the predictions made by TALOS are found to be in error.     

The Catalytic Transition State in ATP Synthase

The catalytic transition state of ATP synthase has been characterized and modeled by combined use of (1) Mg-ADP–fluoroaluminate, Mg-ADP–fluoroscandium, and corresponding Mg-IDP–fluorometals as transition-state analogs; (2) fluorescence signals of -Trp331 and -Trp148 as optical probes to assess formation of the transition state; (3) mutations of critical catalytic residues to determine side-chain ligands required to stabilize the transition state. Rate acceleration by positive catalytic site cooperativity is explained as due to mobility of -Arg376, acting as an arginine finger residue, which interacts with nucleotide specifically at the transition state step of catalysis, not with Mg-ATP- or Mg-ADP-bound ground states. We speculate that formation and collapse of the transition state may engender catalytic site / subunit-interface conformational movement, which is linked to -subunit rotation.     

Adaptive networks using learning matrices

Summary The performance of the Learning Matrix (LM) is suitable for the design of adaptive networks of higher complexity. It has been published, how to connect a LM with a generator of patterns (binary or nonbinary) and a ring-counter to result in an automatic classification of the presented patterns. This paper describes, how to connect two LM's to form an Autonomous Learning Matrix Dipole (ALD) and how to organize it, so that it adapts itself to an environment according to a given evaluation scale. For this purpose, a third type of input (beside e and b), namely h seems to be useful. This h-input controls the rate of adaptation of the LM.Using such ALD's, one may design adaptive structures of even higher complexity, for example with an adaptive internal model.The principle of Learning Matrices has been explained in detail (see e.g. IEEE Transactions on Electronic Computers, Vol. EC-12, No. 6, December, 1963, pp. 846–862). Using such learning matrices (LM), one may build up adaptive networks with rather interesting functions. Perhaps they are interesting for the physiologist and psychologist as well as for the engineer. Let us first recall the most essential details of the LM's.

---

Zusammenfassung Die Funktion der Lernmatrix (LM) erlaubt den Entwurf adaptiver Netzwerke höherer Komplexität. Es wurde an anderer Stelle schon beschrieben, wie eine LM (binär oder nichtbinär) mit einem Generator für Eigenschaftssätze und einem Ringzähler zusammengeschaltet werden kann, um eine selbsttätige Klassifikation der angebotenen Eigenschaftssätze zu bewirken. Im vorliegenden Aufsatz wird erklärt, wie zwei LM so zusammengeschaltet werden können, dacß sich ein Autonomer Lernmatrix-Dipol (ALD) ergibt, und wie dieser zu organisieren ist, daß er sich einer gegebenen Außenwelt nach Maßgabe einer vorgegebenen Werteskala anpaßt. Zu diesem Zweck erweist sich außer den bisher beschriebenen beiden Zugangen zur LM (nämlich e und b) ein dritter sehr zweckmäßig, nämlich h. Dieser h-Eingang beeinflußt die Lerngeschwindigkeit der LM.Unter Verwendung solcher ALD's kann man adaptive Strukturen noch höherer Komplexität aufbauen, beispielsweise solche mit adaptivem innerem Modell.

---

---

Visiting Professor of Electrical Engineering Stanford University.     

Identification and quantitation of adenosine-3′:5′-cyclic monophosphate in plants using gas chromatography-mass spectrometry and high-performance liquid chromatography

Direct evidence has been obtained for the presence of adenosine-3:5-cyclic monophosphate (cAMP) in tobacco (Nicotiana tabacum L.) callus tissue cultures, bean (Phaseolus vulgaris L.) seedlings and immature kernels of sweet corn (Zea mays L.) through the use of a highly specific and sensitive gas chromatography-mass spectrometric assay. Levels of endogenous cAMP ranged from 70 to 126 pmol/g fresh weight. Corresponding levels of cAMP determined for the same samples using radioimmunoassay were consistently three to four times higher. Contrary to previous reports for citrus plants, measurable levels of cAMP could not be detected in young lemon leaves within the limits of detection of the mass-spectrometric assay method. In the case of tobacco callus tissue, the coumarin glucoside, scopolin, which was present in large amounts and showed similar chromatographic behaviour to cAMP, interferred strongly with the mass-spectrometric measurements of cAMP in inadequately purified extracts. The use of high-performance liquid chromatography, in addition to standard chromatographic purification methods, produced highly purified plant extracts for quantitation of cAMP and also provided a method for the separation of cAMP from its 2:3-isomer.Abbreviations cAMP adenosine-3:5-cyclic monophosphate - 2:3-cAMP adenosine-2:3-cyclic monophosphate - GC-MS-MID combined gas chromatography-mass spectrometry with selected multiple-ion-detection - HPLC high-performance liquid chromatography - RIA radioimmunoassay - TLC thin-layer chromatography     

Photosynthetic phosphorylation

A brief history of the discovery of photosynthetic phosphorylation by chloroplasts and bacterial chromatophores is presented. Arnon early introduced the terminology of Cyclic and Non-cyclic photophosphorylation and Cyclic and Non-Cyclic electron transport to the processes observed in illuminated chloroplasts. He made major contributions to the elucidation of these processes and stressed their great biological significance. Investigations of the electron transport components of chromatophores have led to the isolation, purification and crystallization of bacterial reaction centers. The development of three-dimensional molecular structures, and the characterization of their electron transfer components have provided a great deal of information about the early reactions of bacterial photosynthesis. The electron transfer schemes presented clearly support the cyclic nature of light-induced electron transfer. Recent developments in the understanding of ATP synthesis in oxidative phosphorylation by mitochondria and in photophosphorylation by chloroplasts and bacterial chromatophores are discussed.Abbreviations ADP, ATP adenosine 5-di- and triphosphates - NADP⁺, NADPH oxidized and reduced Nicotinamide-adenine dinucleotide phosphate - RC reaction center - EPR electron paramagnetic resonance - F₀F₁ ATP-synthase (synthetase) of mitochondria, chloroplasts, and of chromatophores - F₀ membrane portion of ATP-synthase - F₁-ATPase water soluble sector of ATP-synthase     

Amyloid-Beta Immunization in Alzheimer's Disease Transgenic Mouse Models and Wildtype Mice

Alzheimer's disease is the most prevalent form of dementia worldwide. Therapies are desperately needed to prevent and cure the disease. Mouse models of amyloid- deposition [APP and PSAPP transgenic (tg) mice] have been useful in determining the role of amyloid- (A) in both the pathogenesis and cognitive changes in AD. In addition, they have allowed scientists to investigate potential AD therapies in living animals. Active and passive A immunizations have been employed successfully in APP and PSAPP tg mice to lower cerebral A levels and improve cognition. Optimization of immunization protocols and characterization of immune responses in wildtype mice have been reported. Based on the promising results of A immunization studies in mice, a clinical trial was initiated for A vaccination in humans with AD. Although no adverse effects were reported in the Phase I safety trials, about 5% of AD patients in the phase II clinical trial developed meningoencephalitis, ending the trial prematurely in March 2002. Studies in AD mouse models and wildtype mice may help elucidate the mechanism for these unwanted side effects and will be useful for testing newer, safer vaccines for future use in human clinical trials.     

Zur Histochemie von Hydrolasen im Hoden des Hundes und der Katze

Zusammenfassung Wir untersuchten das Verteilungsmuster von unspezifischer Esterase, alkalischer Phosphatase, Adenosintriphosphatase, 5-Nucleotidase und -D-Glucuronidase im Hoden von Hund und Katze. Besonders hervorzuheben sind eine starke Aktivität der unspezifischen Esterase in den Sertolizellen der Katze, der Reichtum der Membrana propria aller Hodentubuli an alkalischer Phosphatase und Adenosintriphosphatase sowie die kräftige Reaktion auf -D-Glucuronidase in den Leydigzellen beider Tierarten.Die Befunde werden diskutiert.

---

Summary The localization of unspecific esterase, alkaline phosphatase, adenosine triphosphatase, 5-nucleotidase, and -D-glucuronidase in the testes of cat and dog was demonstrated by histochemical means. We observed a strong esterase activity in the Sertoli cells of the cat and high amounts of alkaline phosphatase and adenosine triphosphatase in the membrana propria of all seminiferous tubules. In both species the principal site of -D-glucuronidase was in the Leydig cells. Our findings obtained being discussed.

     

Introduction of foreign genes into potato cultivars Bintje and Désirée using an Agrobacterium tumefaciens binary vector

Tuber discs of Solanum tuberosum cv Bintje and Désirée were cocultivated with an Agrobacterium tumefaciens binary vector, carrying both the neomycine phosphotransferase and the E. coli -glucuronidase gene fused to resp. the nopaline synthase and Cauliflower mosaic virus 35S promotor.Inoculated tuber discs produce transgenic shoots in selective media containing kanamycin. The transgenic plants are phenotypically normal and contain the euploid number of chromosomes. Both the neomycin phosphotransferase as well as the -glucuronidase gene are expressed conferring resp. kanamycin resistance and -glucuronidase activity to the plants.Abbreviations GUS -glucuronidase - NPT neomycin phosphotransferase - CaMV Cauliflower Mosaic Virus - BAP 6-benzylaminopurine - GA₃ gibberellic acid - NAA naphthalineacetic acid - LB Luria Broth - MU methylumbelliferone     

Abbau von 14C-, 3H- und 36Cl-markiertem γ-Hexachlorcyclohexan durch anaerobe Bodenmikroorganismen

Zusammenfassung Durch eine anaerobe Mischflora aus Ackerboden wurde -Hexachlorcyclohexan (-HCH) in 4–5 Tagen zu 90% abgebaut. Dabei erfolgte eine schnelle Abspaltung des Chlors in Form von Chloridionen und danach eine Freisetzung des C- und H-Anteiles in Form flüchtiger Verbindungen, in denen kein Chlor und auch kein CO₂ nachzuweisen war.Die Verwendung von ¹⁴C/³H- und ³⁶Cl/³H-doppelmarkiertem -HCH zeigte, daß die Cl- und H-Abspaltung nicht im Verhältnis von 1:1 erfolgte, sondern mehr Cl als H abgespalten wurde. Die flüchtigen Verbindungen enthielten andererseits höhere ¹⁴C- als ³H-Anteile. Gaschromatographische Untersuchungen zeigten ebenfalls eine rasche Verminderung des -HCH und die Bildung verschiedener Metabolite. Es wurde jedoch kein -Pentachlorcyclohexen nachgewiesen. Bei steigenden O₂-Gehalten in der Gasphase verminderte sich der -HCH-Abbau. Jedoch fanden auch noch bei 5% O₂ Chlorabspaltung und die Freisetzung flüchtiger Metabolite statt.-HCH wurde ebenfalls, jedoch langsamer, durch die anaerobe Mischflora abgebaut. Auch hier wurde Chlorid abgespalten, und es traten ebenfalls flüchtige Verbindungen auf, die kein Chlor enthielten.

---

Degradation of ¹⁴C-, ³H- and ³⁶Cl-labelled -hexachlorocyclohexane by anaerobic soil microorganisms

Up to 90% of the -Hexachlorocyclohexane (-HCH) applied to an anaerobic mixed bacterial flora enriched from an arable soil were degraded within 4–5 days. Degradation resulted in a rapid release of chloride and in formation of chlorine-free volatile metabolites. CO₂ formation from the molecule was not detected.Investigations with ¹⁴C/³H- and ³⁶Cl/³H double-labelled -HCH indicated that the release of Cl and H did not occur in the ratio of 1:1. More Cl than H was split off. The volatile compounds contained more ¹⁴C than ³H. Gas chromatographic studies also showed the rapid decrease of -HCH and the formation of several metabolites. -Pentachlorocyclohexene was not detected. Increasing O₂-contents in the gas phase of cultures resulted in decreases of the compound's degradation. Release of chloride and of volatile metabolites were observed with O₂ contents in the gas phase up to 5%.-HCH was also, but more slowly as with -HCH, degraded by the anaerobic mixed flora. Chloride was released and volatile, chlorine-free metabolites were found.

     

Nucleolar changes in human phytohaemagglutinin-stimulated lymphocytes

Summary The nucleoli of lymphocytes from circulating peripheral blood and from phytohaemagglutinin (PHA)-stimulated cultures (from 2 h–96 h) were studied using a silver method, RNA-specific fluorescent staining, and electron microscopy of ultrathin sections. In peripheral blood about 75% of the lymphocytes have one ring-shaped nucleolus composed of a distinct fibrillar centre surrounded by a dense pars fibrillaris and little granular material; the remaining lymphocytes showing two or more small ring-shaped nucleoli. With PHA stimulation, the number of cells with several nucleoli increases first (from 2 h–12 h). Next, cells containing one or, at most, two large nucleoli with nucleolonema devoid of fibrillar centers are seen (from 4 h on). 34 h after PHA, nucleoli of the compact type containing one or more fibrillar centres appear and comprise about 60% of the cells after 72 h. The appearance of more than one nucleolus per cell shortly after PHA administration suggests an activation of additional nucleolar organizer regions (NOR), which fuse to form one or two large nucleoli with nucleolonema. These are then transformed into compact nucleoli. The fibrillar centers stain preferentially with silver. They contain nonchromosomal proteins and may serve as stores for nucleolar proteins. The fusion of activated NORs during the first cell cycle explains the relatively high frequency of satellite associations in first mitoses compared to later mitoses after stimulation.     

Über das Wachstum der Pankreaszellen von Säugetieren als Monolayer Cultures

Zusammenfassung Glucose und Coffein erhöhen den Gehalt 4 und 7 Tage alter Zellen an immunologisch meßbarem Insulin (Ausgangsmaterial: Ratten- und Schweinepankreas). Morphologisch (Aldehydfuchsin, Pseudoisocyanin) sind bei coffeinbehandelten Zellen in der Intensität der Anfärbung und in der Granuladichte zeitabhängige Unterschiede zu beobachten, die an 4 Tage alten Zellen deutlicher als an 7 Tage alten zu erkennen sind. Coffein erhöht die Verfettung der Zellen. Weiter nimmt der Gehalt an sauren Mucopolysacchariden (Eisenbindungsreaktion) und an PAS-positivem Material zu. Diese Erhöhung läuft mit dem Anstieg des Insulingehaltes im Nährmedium parallel.

---

Monolayer cultures of pancreatic tissueIII. Insulin release induced by coffein and glucose

Summary Glucose and caffeine increase the immunologically measurable insulin content of four and seven-day old cells (starting material: rats' or pigs' pancreas). In morphological examination (aldehyde fuchsin, pseudoisocyanin), time-dependent differences in the intensity of staining and granular density are observable in caffeine-treated cells; these phenomena are more distinct in four-day old cells than in seven-day old ones. Caffeine increases fatty degeneration of the cells. Furthermore, the content of acid mucopolysaccharides (iron-binding reaction) and of PAS positive material increases. This increase runs parallel with the rise in insulin content of the nutritive medium.

     

“Primäre” und “Sekundäre” Differenzierung im Zusammenhang mit der Photomorphogenese von Keimpflanzen (Sinapis alba L.)

Zusammenfassung Die Anthocynsyanthese des Senfkeimlings ist phytochromabhängig. Lediglich zwei Gewebe, die Epidermis der Cotyledonen und die Subepidermis des Hypocotyls sind zu dieser Anthocyansynthese fähig. Erst 24 Std nach Aussaat ist Anthocyansynthese möglich und bereits etwa 60 Std nach Aussaat (25° C; Standardbedingungen vgl. Methoden) erlischt dei Fähigkeit zur Anthocyansynthese weitgehend und zwar unabhängig von der Menge des synthetisierten Anthocyans. Die höchste Empfindlichkeit für Licht besitzt das Anthocyan bildende System etwa 36 Std nach Aussaat. — Teilt man den Keimling unmittelbar vor der Anthocyanmessung in 4 Segmente auf (Abb. 9) und mißt den Anthocyangehalt der Segmente getrennt, so stellt sich heraus, daß die Fähigkeit zur Anthocyansynthese im mittleren und basalen Bereich des Hypocotyls rapide verloren geht. Im oberen Hypocotylabschnitt hingegen und in den Cotyledonen nimmt diese Fähigkeit erst zu, und die Abnahme ist langsamer. —Es werden Argumente für die Auffassung entwickelt, daß das spezifische und dynamische Zellmuster, das man hinsichtlich der P₇₃₀-abhängigen Anthocyansynthese vorfindet, ein Ausdruck der primären Differenzeierung sei (vgl. Abb. 4). P₇₃₀ hingegen, so stellen wir uns vor, wirkt unspezifisch im Rahmen einer sekundären Differenzierung, indem es potentiell aktive Gene (P₇₃₀) in Funktion setzt. Welche Gene in den einzelnen Zellen des Dunkelkeimlings potentiell aktiv sind, legt die primäre Differenzierung fest. — Diese Vorstellungen werden durch den Befund gestützt, daß eine Applikation von Actinomycin D zu einer zeitlich sehr viel ausgedehnteren Anthocyansynthese führt; offenbar deshalb, weil die genetisch kontrollierte Entwicklung des primären Differenzie-rungsmusters gebremst wird. Eine Folge wäre, daß die Inaktivierung der zur Anthocyansynthese benötigten Gene, die normalerweise etwa 60 Std nach Aussaat erfolgt, weit hinausgezögert wird.

---

Primary and secondary differentiation in connection with photomorphogenesis of seedlings (Sinapis alba L.)

Summary Anthocyanin synthesis of the mustard seedling (Sinapis alba L.), a typical phytochrome-dependent photoresponse has been further investigated. — It has been found that only two types of tissue can synthesize anthocyanin under the influence of active phytochrome (=P₇₃₀), namely, the epidermis of the votyledons and the subepidermal layer in the hypocotyl (Fig. 2, 3). — Under our standard conditions (25° C; cf. methods) phytochrome-potentiated anthocyanin synthesis is only possible 24 hours after sowing and it ceases about 60 hours after sowing, independent of the amount of anthocyanin which has been accumulated (Fig. 5, 6). On the basis of the whole seedling the highest sensitivity of the anthocyanin producing system to light is around 36 hours after sowing (Fig. 8). Within the tissues which are capable of forming anthocyanin there is a characteristic shift of the ability to respond to P₇₃₀ as the seedling ages. If we devide the seedling into 4 segments (Fig. 9) it turns out that in the basal and middle part of the hypocotyl the ability to form anthocyanin is rapidly lost whereas in the upper part of the hypocotyl and in the cotyledons this ability even increases at first. The following decrease is slower than in the basal parts (Fig. 10, 11).It is argued that this specific and dynamic cellular pattern of responsiveness to P₇₃₀ can be regarded as a manifestation of a primary differentiation in the course of which the genotype of each individual cell in the dark-grownt seedling is devided into 3 functional types of genes: active, inactive, and potentially active genes (P₇₃₀) (Fig. 4). — In connection with anthocyanin synthesis P₇₃₀ is thought to act exclusively at the level of secondary differentiation, i.e., it is thought to initiate the action of potentially active genes via a signal-chain. The action of P₇₃₀ is non-specific. The specificity of the photoresponse of an individual cell is determined by the status of its primary differentiation (Fig. 4).If the process of differentiation is slowed down (e.g. by the application of low doses of Actiomycin D) anthocaynin synthesis can continue much longer than under our standard conditions where it ceases around 60 hours after sowing (Fig. 12). This fact seems to indicate that the loss of the ability to form anthocyanin is due to an inactivation of pertinent genes by the process of primary differentiation, which is itself, as one would expect, under the control of genes.

     

Primary structure of hemoglobin β-chain fromColumba livia (gray wild pigeon)

Primary structure of -chain of pigeon is presented. It was determined by amino acid sequence analysis of intact -chain and its peptides obtained by the enzymatic and chemical cleavage. Comparison of amino acid sequence of the chain with other available data shows 14 Ile, 61 Lys, and 113 Ile as residues specific to pigeon. One important replacement at ₁₁ contact is 55 MetSer.     

New genetic variants identified in donkey's milk whey proteins

Novel genetic variants for donkey milk lysozyme and -lactoglobulins I and II have been identified by the combined use of peptide mass mapping and sequencing by tandem mass spectrometry in association with database searching. The novel donkey lysozyme variant designated as lysozyme B (Mr 14,631 Da) differed in three amino acid exchanges, N⁴⁹ D, Y⁵² S, and S⁶¹ N, from the previously published sequence. Three novel genetic variants for donkey -lactoglobulins were identified. One of them is a type -lactoglobulin I with three amino acid exchanges at E³⁶ S, S⁹⁷ T, and V¹⁵⁰ I (-lactoglobulin I B, Mr 18,510 Da). The two others are type -lactoglobulins II with two amino acid exchanges at C¹¹⁰ P and M¹¹⁸ T (-lactoglobulin II B, Mr 18,227 Da) and with three amino acid exchanges at D⁹⁶ E, C¹¹⁰ P, and M¹¹⁸ T (-lactoglobulin II C, Mr 18,241 Da). All these primary structures are closely related to those of homologous proteins in horse milk (percent identity >96%).     

In vitro culture ofXanthium strumarium (Cocklebur)

Xanthium strumarium L. was micropropagated by rooting shoots proliferated from shoot-tip explants. The best shoot proliferation was obtained from explants growing on Murashige and Skoog medium supplemented with 4.4 to 8.9 M benzyladenine (BA) and 1.1 to 2.1 M naphthaleneacetic acid (NAA). The micropropagated plants were transferred to potting media and maintained under high humidity conditions in the greenhouse. The media that produced best shoot proliferation from shoot-tip explants also produced the most callus from hypotocotyl, cotyledon and shoot-tip explants, whereas more callus was produced on leaf explants with a lower BA concentration (1.1 M) and 1.1 M NAA.Abbreviations BA benzyladenine, 2 4-d-2,4-dichlorophenoxyacetic acid - IAA indole-3-acetic acid - NAA naphthaleneacetic acid - MS Murashige and Skoog Technical contribution No. 3319 of the South Carolina Agricultural Experiment Station, Clemson University.