Social Behaviour on the Wing in the False Vampire,Megaderma lyra

Social interaction occurs in bats. In a group of 10 Megaderma lyra (seven female and two male adults, as well as one female juvenile) held in captivity, two stereotyped flying behaviour patterns —the ‘grumbling flight’ and the ‘song flight’ — were observed and studied. The ‘grumbling flight’ is a social interaction in flight between at least two Megaderma lyra in which ‘grumble sequences’ are emitted. This behaviour is triggered by stress or arising aggression, and presumably attempts to avoid agonistic interactions with dangerous physical contact. The song flight was exclusively displayed by the dominant male bat and only directed at the non-lactating female members of the group, with a preference to alien females. This behaviour is composed of three behavioural stages, each accompanied by a specific ‘song strophe’. The song flight presumably aims at bonding the females to the male. During the grumbling flight and the song flight, M. lyra emits communication sounds in the ultrasonic range. The sounds consist of simple elements (FM_down, FM_up, CF), and are similar to types of sounds emitted for echolocation by various bat species.     

Lymphoid malignancies: the dark side of B-cell differentiation

When the regulation of B-cell differentiation and activation is disrupted, lymphomas and leukaemias can occur. The processes that normally create immunoglobulin diversity might be misdirected, resulting in oncogenic chromosomal translocations that block differentiation, prevent apoptosis and/or promote proliferation. Prolonged or unregulated antigenic stimulation might contribute further to the development and progression of some malignancies. Lymphoid malignancies often resemble normal stages of B-cell differentiation, as shown by molecular techniques such as gene-expression profiling. The similarities and differences between malignant and normal B cells indicate strategies for the treatment of these cancers.     

Multistability: a major means of differentiation and evolution in biological systems.

Very simple biochemical systems regulated at the level of gene expression or protein function are capable of complex dynamic behaviour. Among the various patterns of regulation associated with non-linear kinetics, multistability, which corresponds to a true switch between alternate steady states, allows a graded signal to be turned into a discontinuous evolution of the system along several possible distinct pathways, which can be either reversible or irreversible. Multistability plays a significant role in some of the basic processes of life. It might account for maintenance of phenotypic differences in the absence of genetic or environmental differences, as has been demonstrated experimentally for the regulation of the lactose operon in Escherichia coli. Cell differentiation might also be explained as multistability.     

Possible molecular mechanisms of the protonmotive function of cytochrome systems.

The object of this paper is to help to evolve a conceptual framework suitable for exploring and explaining the mechanisms of protonmotive cytochrome systems.A review of some of the knowledge of the kinetic and equilibrium behaviour of the classical cytochrome systems of mitochondria indicates that the simple redox loop concept is not adequate for building a realistic conceptual model. In particular, the remarkable behaviour of the components of the cytochrome b-c₁ complex, which has long been regarded as puzzling, cannot be explained on the basis of simple redox loop formulations. However, the newly introduced concepts of the protonmotive ubiquinone cycle, or Q cycle, and of the cyclic loop 2–3 system, which represent developments of the redox loop concept, are shown to provide a promising basis for the evolution of a satisfactory theory.The mechanism of the Q cycle is discussed and developed in the light of experimental knowledge of classical mitochondrial cytochrome systems. The possible operation of a Q cycle in chloroplasts and bacteria is briefly discussed, and attention is drawn to bacterial cytochrome systems that appear to be organized as simple redox loops rather than as cyclic systems.Some aspects of notions of direct chemiosmotic coupling and indirect conformational coupling are compared in the context of research strategy.     

A propionate CoA-transferase of Ralstonia eutropha H16 with broad substrate specificity catalyzing the CoA thioester formation of various carboxylic acids

In this study, we have investigated a propionate CoA-transferase (Pct) homologue encoded in the genome of Ralstonia eutropha H16. The corresponding gene has been cloned into the vector pET-19b to yield a histidine-tagged enzyme which was expressed in Escherichia coli BL21 (DE3). After purification, high-performance liquid chromatography/mass spectrometry (HPLC/MS) analyses revealed that the enzyme exhibits a broad substrate specificity for carboxylic acids. The formation of the corresponding CoA-thioesters of acetate using propionyl-CoA as CoA donor, and of propionate, butyrate, 3-hydroxybutyrate, 3-hydroxypropionate, crotonate, acrylate, lactate, succinate and 4-hydroxybutyrate using acetyl-CoA as CoA donor could be shown. According to the substrate specificity, the enzyme can be allocated in the family I of CoA-transferases. The apparent molecular masses as determined by gel filtration and detected by SDS polyacrylamide gel electrophoresis were 228 and 64 kDa, respectively, and point to a quaternary structure of the native enzyme (α₄). The enzyme exhibited similarities in sequence and structure to the well investigated Pct of Clostridium propionicum. It does not contain the typical conserved (S)ENG motif, but the derived motif sequence EXG with glutamate 342 to be, most likely, the catalytic residue. Due to the homo-oligomeric structure and the sequence differences with the subclasses IA–C of family I CoA-transferases, a fourth subclass of family I is proposed, comprising — amongst others — the Pcts of R. eutropha H16 and C. propionicum. A markerless precise-deletion mutant R. eutropha H16?pct was generated. The growth and accumulation behaviour of this mutant on gluconate, gluconate plus 3,3′-dithiodipropionic acid (DTDP), acetate and propionate was investigated but resulted in no observable phenotype. Both, the wild type and the mutant showed the same growth and storage behaviour with these carbon sources. It is probable that R. eutropha H16 is upregulating other CoA-transferase(s) or CoA-synthetase(s), thereby compensating for the lacking Pct. The ability of R. eutropha H16 to substitute absent enzymes by isoenzymes has been already shown in different other studies in the past.     

Myasthenic nicotinic receptor mutant interpreted in terms of the allosteric model

An extended Monod—Wymctn—Changeux allosteric-type model is applied to human muscle nicotinic acetylcholine receptors expressed in HEK cells, for both the normal form and the high-affinity human myasthénic mutant, ε T264P. The model is based on a concerted transition between the basal (resting) B state and the active (open-channel) A state, with the equilibrium in the absence of ligand determined by the allosteric constant, L_o = [B₀]/[A₀]. For wild-type receptors the model with L₀ = 910⁸ provides a satisfactory representation of published patch-clamp recordings that yields a distribution of open-channel dwell times with a single peak at 0.7 ms. For the εT264P mutant, the model with L₀ = 100 accounts for the trimodal distribution reported for open-channel dwell times, with peaks at 0.15, 3.8 and 60 ms that correspond to non-, mono- and bi-liganded receptors, respectively. Possible applications of the allosteric model to other myasthénic mutants are considered.     

Boolean analysis of cell regulation networks

A comparison is made between the predictions of the Boolean and continuous analysis of a regulation model when the formation of two mediators interacting by cross-inhibition is stimulated by one or two specific signals. For such a system, the Boolean analysis reproduces the characteristics of behaviour previously predicted by continuous analysis (multiple stable states of opposite type, discontinuous transition, and associated hysteresis phenomenon). The qualitative agreement between the two methods allows a qualitative but rigorous treatment of regulation systems in which the Boolean analysis is applicable. From a general schematic representation of interaction in bidirectional control systems, we analyse by the Boolean method a large range of possible systems of increasing complexities which could theoretically apply. Previously unforeseen consequences of some systems are described. After that, we give a logical analysis of a well-known system (negative loop grafted with additional external controls) and discuss the application of such a system to explain certain oscillatory phenomena in the cell, showing the disrupting role of an additional control on the expected behaviour. Thus, when the analysis of a model including a negative loop does not indicate the possibility of experimentally suggested oscillations, we propose other simple logical structures which can predict this behaviour. Finally, we show a logical analysis of an opposite type of example of cell regulation where the biochemical observations can be accounted for simply by a negative loop grafted with one input variable.     

高等植物尿素代谢及转运的分子机理

尿素广泛存在于自然界中, 是易于被许多生物(如植物)利用的生长氮源。该文通过概述尿素在不同生命系统中存在的基础生理意义及各类型尿素转运蛋白, 讨论了植物细胞中尿素合成与分解的各种途径及尿素在植物氮营养、代谢和运输中的生理作用。迄今为止, 在植物中已发现了2类转运尿素的膜蛋白, 即MIPs和DUR3, 它们分别在低亲和力、高亲和力尿素运输中发挥潜在作用。异源表达结果表明, MIPs介导了尿素的被动迁移; 而AtDUR3则参与拟南芥根系对尿素的吸收。对MIPs和DUR3转运尿素的酶学特征、亚细胞作用位点和表达调控状况等的研究表明: 它们的分子生物学功能与植物的氮营养及氮素再分配和利用相关。     

高等植物尿素代谢及转运的分子机理

尿素广泛存在于自然界中,是易于被许多生物（如植物）利用的生长氮源。该文通过概述尿素在不同生命系统中存在的基础生理意义及各类型尿素转运蛋白,讨论了植物细胞中尿素合成与分解的各种途径及尿素在植物氮营养、代谢和运输中的生理作用。迄今为止,在植物中已发现了2类转运尿素的膜蛋白,即MIPs和DUR3,它们分别在低亲和力、高亲和力尿素运输中发挥潜在作用。异源表达结果表明MIPs介导了尿素的被动迁移：而AtDUR3则参与拟南芥根系对尿素的吸收。对MIPs和DUR3转运尿素的酶学特征、亚细胞作用位点和表达调控状况等的研究表明：它们的分子生物学功能与植物的氮营养及氮素再分配和利用相关。     

Characterization of a Sorghum bicolor gene family encoding putative protein kinases with a high similarity to the yeast SNF1 protein kinase

C₄ photosynthesis is functionally dependent on metabolic interactions between mesophyll and bundle-sheath cells. Although the C₄ cycle is biochemically well understood many aspects of the regulation of enzyme activities, gene expression and cell differentiation are elusive.Protein kinases are likely involved in these regulatory processes providing links to hormonal, metabolic and developmental signal transduction pathways. We have identified several protein kinases that are differentially expressed in mesophyll and bundle-sheath cells of the C₄ plant Sorghum bicolor. Here we describe the characterization of two putative protein kinases that show high similarity to the SNF1/AMPK family of protein serine/threonine kinases. The mRNA of both kinases accumulates to much higher levels in mesophyll cells than in the bundle-sheath and can also be detected in root tissue. Complementation experiments with a snf1 mutant of Saccharomyces cerevisiae indicate that the S. bicolor protein kinase SNFL1 does not represent a functional homologue of the yeast SNF1 protein kinase.     

The back and forth of energy transfer between carotenoids and chlorophylls and its role in the regulation of light harvesting

Many aspects in the regulation of photosynthetic light-harvesting of plants are still quite poorly understood. For example, it is still a matter of debate which physical mechanism(s) results in the regulation and dissipation of excess energy in high light. Many researchers agree that electronic interactions between chlorophylls (Chl) and certain states of carotenoids are involved in these mechanisms. However, in particular, the role of the first excited state of carotenoids (Car S₁) is not easily revealed, because of its optical forbidden character. The use of two-photon excitation is an elegant approach to address directly this state and to investigate the energy transfer in the direction Car S₁ → Chl. Meanwhile, it has been applied to a large variety of systems starting from simple carotenoid–tetrapyrrole model compounds up to entire plants. Here, we present a systematic summary of the observations obtained by two-photon excitation about Car S₁ → Chl energy transfer in systems with increasing complexity and the correlation to fluorescence quenching. We compare these observations directly with the energy transfer in the opposite direction, Chl → Car S₁, for the same systems as obtained in pump-probe studies. We discuss what surprising aspects of this comparison led us to the suggestion that quenching excitonic Car–Chl interactions could contribute to the regulation of light harvesting, and how this suggestion can be connected to other models proposed.     

DNA methylation profiling distinguishes three clusters of breast cancer cell lines

Methylation change plays an important role in many cellular systems, including cancer development. During recent years, genome-wide or large-scale methylation data has become available thanks to rapid advances in high-throughput biotechnologies. So far, researchers have always used gene expression profiling to study disease subtypes and related therapies. In this study, we investigated methylation profiles in 30 breast cancer cell lines using methylation data generated by microarray technologies. Strong variation of the number of methylation peaks was found among these 30 cell lines; however, more peaks were found in the upstream regions than in downstream regions of genes. We further grouped the methylation profiles of these cell lines into three consensus clusters. Finally, we performed an integrative analysis of breast cancer cell lines using both methylation and gene-expression profiling data. There was no significant correlation between methylation-profiling subtypes and gene-expression profiling subtypes, suggesting the complex nature of methylation in the regulation of gene expression. However, we found basal B cell lines appeared exclusively in two methylation clusters. Although these results are preliminary, this study suggests that methylation profiling might be promising in disease subtype classification and the development of therapeutic strategies.     

Temporal competition between differentiation programs determines cell fate choice

Multipotent differentiation, where cells adopt one of several possible fates, occurs in diverse systems ranging from bacteria to mammals. This decision‐making process is driven by multiple differentiation programs that operate simultaneously in the cell. How these programs interact to govern cell fate choice is poorly understood. To investigate this issue, we simultaneously measured activities of the competing sporulation and competence programs in single Bacillus subtilis cells. This approach revealed that these competing differentiation programs progress independently without cross‐regulation before the decision point. Cells seem to arrive at a fate choice through differences in the relative timing between the two programs. To test this proposed dynamic mechanism, we altered the relative timing by engineering artificial cross‐regulation between the sporulation and competence circuits. Results suggest a simple model that does not require a checkpoint or intricate cross‐regulation before cellular decision‐making. Rather, cell fate choice appears to be the outcome of a ‘molecular race’ between differentiation programs that compete in time, providing a simple dynamic mechanism for decision‐making.     

Mutagenesis of the blue-green alga,Anabaena doliolum Bharadwaja

Mutagenesis in the blue-green alga, Anabaena doliolum Bharadwaja has been investigated with particular reference to N₂ fixation. Several types of mutant have been isolated after induction with UV, NG, acridine orange and acriflavine. From a comparative characterization it is concluded that the heterocyst is not the sole site of N₂ fixation. There does not appear to be a linkage between N₂ fixation and heterocyst or spore differentiation: they seem to be independent processes probably regulated either by different genes or by a single regulatory gene with independent operons. A common genetic determinant has also been suggested for nitrogenase and nitrate and nitrite reductases.     

Combined histomorphometric and gene-expression profiling applied to toxicology

We have developed a unique methodology for the combined analysis of histomorphometric and gene-expression profiles amenable to intensive data mining and multisample comparison for a comprehensive approach to toxicology. This hybrid technology, termed extensible morphometric relational gene-expression analysis (EMeRGE), is applied in a toxicological study of time-varied vehicle- and carbon-tetrachloride (CCl₄)-treated rats, and demonstrates correlations between specific genes and tissue structures that can augment interpretation of biological observations and diagnosis.