DNA Packaging-Associated Hyper-Capsid Expansion of Bacteriophage T3

Evidence that in vivo bacteriophage T3 DNA packaging includes capsid hyper-expansion that is triggered by lengthening of incompletely packaged DNA (ipDNA) is presented here. This evidence includes observation that some of the longer ipDNAs in T3-infected cells are packaged in ipDNA-containing capsids with hyper-expanded outer shells (HE ipDNA-capsids). In addition, artificially induced hyper-expansion is observed for the outer shell of a DNA-free capsid. Detection and characterization of HE ipDNA-capsids are based on two-dimensional, non-denaturing agarose gel electrophoresis, followed by structure determination with electron microscopy and protein identification with SDS-PAGE/mass spectrometry. After expulsion from HE ipDNA-capsids, ipDNA forms sharp bands during gel electrophoresis. The following hypotheses are presented: (1) T3 has evolved feedback-initiated, ATP-driven capsid contraction/hyper-expansion cycles that accelerate DNA packaging when packaging is slowed by increase in the packaging-resisting force of the ipDNA and (2) each gel electrophoretic ipDNA band reflects a contraction/hyper-expansion cycle.     

The Evolution of Control and Distribution of Adaptive Mutations in a Metabolic Pathway

In an attempt to understand whether it should be expected that some genes tend to be used disproportionately often by natural selection, we investigated two related phenomena: the evolution of flux control among enzymes in a metabolic pathway and properties of adaptive substitutions in pathway enzymes. These two phenomena are related by the principle that adaptive substitutions should occur more frequently in enzymes with greater flux control. Predicting which enzymes will be preferentially involved in adaptive evolution thus requires an evolutionary theory of flux control. We investigated the evolution of enzyme control in metabolic pathways with two models of enzyme kinetics: metabolic control theory (MCT) and Michaelis–Menten saturation kinetics (SK). Our models generate two main predictions for pathways in which reactions are moderately to highly irreversible: (1) flux control will evolve to be highly unequal among enzymes in a pathway and (2) upstream enzymes evolve a greater control coefficient then those downstream. This results in upstream enzymes fixing the majority of beneficial mutations during adaptive evolution. Once the population has reached high fitness, the trend is reversed, with the majority of neutral/slightly deleterious mutations occurring in downstream enzymes. These patterns are the result of three factors (the first of these is unique to the MCT simulations while the other two seem to be general properties of the metabolic pathways): (1) the majority of randomly selected, starting combinations of enzyme kinetic rates generate pathways that possess greater control for the upstream enzymes compared to downstream enzymes; (2) selection against large pools of intermediate substrates tends to prevent majority control by downstream enzymes; and (3) equivalent mutations in enzyme kinetic rates have the greatest effect on flux for enzymes with high levels of flux control, and these enzymes will accumulate adaptive substitutions, strengthening their control. Prediction 1 is well supported by available data on control coefficients. Data for evaluating prediction 2 are sparse but not inconsistent with this prediction.THEORETICAL research on the process of adaptation has focused primarily on describing the size and number of genetic changes underlying phenotypic change (Fisher 1930; Kimura 1983; Orr 1998, 2002, 2003). By contrast, comparatively little theoretical attention has been given to the question of whether certain genes or types of genes are preferentially involved in the process of adaptation. Yet the current debate over the relative importance of regulatory vs. structural genes in morphological evolution (Hoekstra and Coyne 2007; Stern and Orgogozo 2008) clearly indicates that this question is of interest to evolutionary biologists.One situation in which this question is pertinent is the evolution of characters that are influenced by the concentration of end products of metabolic pathways. Often change in end-product concentration can be achieved by substitutions in any one of several genes in the pathway. One example is the intensity of floral pigmentation. To a first approximation, final pigment concentration, and hence color intensity, can be viewed as being determined by the flux rate down the pigment biosynthetic pathway for a fixed time corresponding to the duration of floral development. More generally, any situation in which flux rate determines phenotype is likely to fall in this category. In such situations, metabolic control theory (MCT) (Kacser and Burns 1973) and similar approaches (Heinrich and Rapoport 1974; Savageau 1976) indicate that changes in flux can be achieved by changing the activity of any enzyme in the pathway. We seek to determine whether and, if so, why enzymes differ in the probability that they contribute to evolutionary change in pathway flux.It has been suggested as a general principle that enzymes with the greatest control over flux will be disproportionately involved in such evolutionary change (Hartl et al. 1985; Eanes 1999; Watt and Dean 2000). This argument is based on the theoretical expectation that the probability of fixation of an advantageous allele is roughly proportional to its selection coefficient (Hedrick 2000). Since mutations equivalent in terms of enzyme kinetic properties will have greater effects on flux, and hence on fitness, in enzymes with greater metabolic control, mutations in those enzymes will be substituted preferentially.While this argument is likely sound, it simply pushes back the question of which genes evolve preferentially to the question of which enzymes are expected to have greatest control over flux. Although we are unaware of any theoretical attempts to model the evolution of flux control, many authors have speculated about where in pathways control is expected to be highest.Kacser and Burns (1973) hypothesized that the magnitudes of flux control exerted by different enzymes may be very similar. This hypothesis was based on the result from MCT that in linear pathways, overall flux control can be shared by all enzymes. Since metabolic pathways often consist of many enzymes, each would be expected to have only a limited potential to influence flux. Subsequent theoretical analysis of this hypothesis demonstrated that a given flux is consistent with many different flux-control distributions, including, at one extreme, equal flux control by all enzymes and, at the other extreme, major control by one or a few enzymes and little control for all others (Mazat et al. 1996). However, the question of which of these possibilities, if any, are likely to be favored by selection has not been addressed.Another hypothesis, the epistatic or synergistic principle, predicts that control will be vested in a single enzyme at any given time, but will shift over time among enzymes (Dykhuizen et al. 1987; Keightley 1989; Bost et al. 2001) According to this hypothesis, starting from equal control among enzymes in the pathway, selection to increase (or decrease) flux will cause the activity of one enzyme to increase (decrease). This change results in a decrease (increase) in flux control for the enzyme that changes and an increase (decrease) in control for the other pathway enzymes, causing control to be unequally shared. While this argument seems plausible, there has been no analysis of whether over time all enzymes have an equal chance of having elevated control.Finally, Eanes'' (1999) review of enzyme polymorphisms found that control is often centered in enzymes at pathway branch points, which constitute the most upstream enzymes of their specific branch. Flowers et al. (2007) also demonstrated that branching enzymes tend to exhibit more adaptive substitutions than downstream enzymes as would be expected under the principle that evolutionary change will be concentrated in enzymes with the largest control coefficients. In addition, evolutionary changes in these enzymes may be favored because they allow organisms to modify flux allocation to alternate functions and track environmental fluctuations. This suggestion is supported by the “branch point effect,” a theoretical demonstration that control coefficients can dramatically shift between enzymes depending on the kinetic rates of the two competing enzymes (LaPorte et al. 1984). However, this study does not address the question of how the distribution of control is likely to evolve, but describes only which distributions of control are mathematically possible. Thus, Eanes (1999, p. 318) concludes his review, stating “all enzymes in [a] contributing pathway may not be equal; determining the rule[s] for these inequalities should be a major goal in studies of enzyme polymorphism.”A control coefficient (CC) indicates the degree to which flux through a pathway is altered by a small change in the activity of an enzyme (see appendix; this is equivalent to the sensitivity coefficient of Kacser and Burns 1973). The “rules” governing the distribution of control coefficients are determined by the biological evolution of metabolic systems. While research demonstrates that there are many possible distributions of control coefficients, none has examined which of these is most likely to evolve. The optimization of metabolic systems has been explored in detail (Heinrich et al. 1991, 1997; Heinrich and Schuster 1998). In these studies, however, the investigators employ as optimization criteria maximizing flux, maximizing transient times, or minimizing metabolic intermediates, criteria whose biological and evolutionary relevance is unclear.In an effort to understand how control is expected to be shared among enzymes and predict which enzymes are most likely to contribute to adaptive genetic changes, we present two models of the evolution of flux control in a simple linear pathway. The first model employs the framework of MCT. Although there have been many challenges to the MCT framework (Savageau 1976, 1992; Cornish-Bowden 1989; Savageau and Sorribas 1989), it should be made clear that our aim is not to construct a precisely parameterized model of a particular biological system, but to use this generalized framework to address a single, critically ignored question: What are the rules governing how control will evolve to be distributed among enzymes? The use of the MCT framework to address questions in evolutionary genetics is firmly established, with investigation focused on the molecular basis of dominance (Kacser and Burns 1981; Keightley 1996a; Phadnis and Fry 2005; but see Bagheri and Wagner 2004), the relationship between metabolic flux and fitness (Dykhuizen et al. 1987; Szathmary 1993), the amount of additive and nonadditive genetic variance in metabolic systems (Keightley 1989), whether this variation can be explained by mutation–selection balance (Clark 1991), and patterns of response of quantitative traits to selection (Keightley 1996b). The second model we examine, saturation kinetics (SK), is based on Michealis–Menten kinetics and enables us to relax one major assumption of MCT: that enzymes are far from saturation.Here we limit our analysis to linear pathways as an initial attempt to examine these issues. We find that for such pathways control coefficients will generally evolve to be unequal; that the magnitude of this inequality depends on the thermodynamic properties, rather than the kinetic properties, of each reaction step; that upstream enzymes tend to evolve higher control coefficients than downstream enzymes; and that upstream enzymes fix advantageous mutations in greater numbers, and those mutations have larger effects than in downstream enzymes.     

Bacterial Evolutionary Precursors of Eukaryotic Copper–Zinc Superoxide Dismutases

Internalization of a bacteria by an archaeal cell expedited eukaryotic evolution. An important feature of the species that diversified into the great variety of eukaryotic life visible today was the ability to combat oxidative stress with a copper–zinc superoxide dismutase (CuZnSOD) enzyme activated by a specific, high-affinity copper chaperone. Adoption of a single protein interface that facilitates homodimerization and heterodimerization was essential; however, its evolution has been difficult to rationalize given the structural differences between bacterial and eukaryotic enzymes. In contrast, no consistent strategy for the maturation of periplasmic bacterial CuZnSODs has emerged. Here, 34 CuZnSODs are described that closely resemble the eukaryotic form but originate predominantly from aquatic bacteria. Crystal structures of a Bacteroidetes bacterium CuZnSOD portray both prokaryotic and eukaryotic characteristics and propose a mechanism for self-catalyzed disulfide maturation. Unification of a bacterial but eukaryotic-like CuZnSOD along with a ferredoxin-fold MXCXXC copper-binding domain within a single polypeptide created the advanced copper delivery system for CuZnSODs exemplified by the human copper chaperone for superoxide dismutase-1. The development of this system facilitated evolution of large and compartmentalized cells following endosymbiotic eukaryogenesis.     

Heritability and genetic covariation of sensitivity to PROP, SOA, quinine HCl, and caffeine

The perceived bitterness intensity for bitter solutions of propylthiouracil (PROP), sucrose octa-acetate (SOA), quinine HCl and caffeine were examined in a genetically informative sample of 392 females and 313 males (mean age of 17.8 +/- 3.1 years), including 62 monozygotic and 131 dizygotic twin pairs and 237 sib pairs. Broad-sense heritabilities were estimated at 0.72, 0.28, 0.34, and 0.30 for PROP, SOA, quinine, and caffeine, respectively, for perceived intensity measures. Modeling showed 1) a group factor which explained a large amount of the genetic variation in SOA, quinine, and caffeine (22-28% phenotypic variation), 2) a factor responsible for all the genetic variation in PROP (72% phenotypic variation), which only accounted for 1% and 2% of the phenotypic variation in SOA and caffeine, respectively, and 3) a modest specific genetic factor for quinine (12% phenotypic variation). Unique environmental influences for all four compounds were due to a single factor responsible for 7-22% of phenotypic variation. The results suggest that the perception of PROP and the perception of SOA, quinine, and caffeine are influenced by two distinct sets of genes.     

Sensitizer-mediated photooxidation of histidine residues: evidence for the formation of reactive side-chain peroxides

Exposure of proteins to visible light in the presence of a sensitizer results in the oxidation of Met, Trp, Tyr, Cys, and His side chains. These reactions are only partially understood, particularly with His. In this study, the oxidation of free His, His derivatives, and His-containing peptides has been examined using visible light and a range of sensitizers. It is shown that photooxidation gives rise to unstable peroxides, in a light-, illumination time-, and sensitizer-dependent manner. The yield of these materials is increased when reactions are carried out in solutions prepared with D2O, which prolongs the lifetime of 1O2, and decreased in the presence of the potent 1O2 scavenger azide, consistent with the involvement of this excited state. These peroxides have half-lives of hours, though the rate of decomposition is enhanced by elevated temperatures, reductants, and metal ions. Reducing metal ions catalyze the formation of radicals, which have been detected by EPR spin trapping. Structural analysis of His photo-products using NMR spectroscopy has provided evidence for the formation of oxygenated and cyclized compounds (e.g., 6a-hydroxy-2-oxo-octahydro-pyrollo[2,3-d]imidazole-5-carboxylic acid) and cross-linked materials. The latter materials may be partly responsible for the high yield of aggregated materials detected on photooxidation of His-containing proteins.     

Elevational gradients during the Late-Glacial/Holocene vegetational transition in southern Bulgaria

The Late Glacial and early-Holocene vegetational history of a newly dated pollen and macrofossil diagram from Besbog, a cirque lake at 2250 m just above the forest limit in the Pirin Mountains of southwestern Bulgaria, is compared with a newly dated pollen diagram for the mire Shiroka Polyana at 1400 m in the conifer forest of the nearby Rhodope Mountains in order to investigate the chronology of major changes in the vegetation at different elevations. In the Lake Besbog record the non-arboreal pollen assemblage of the Late Glacial changed abruptly to that of Betula, Quercus and other deciduous types. The date for this change is about 11.6 ka cal b.p. The Quercus assemblage may be composed of pollen blown from intermediate elevations, to which deciduous forest had expanded because of higher summer temperatures related to high summer insolation. At Shiroka Polyana (1400 m) in the modern conifer belt, a similar change did not occur until about 8.8 ka cal b.p. The persistence of the dry steppe or steppe forest in the early Holocene at this lower site can also be attributed to high summer insolation. Thus as atmospheric temperature increased at the end of the Late Glacial, deciduous forests expanded first at intermediate elevations in the Pirin Mountains and only later in the Rhodope Mountains at lower elevations as summer insolation decreased.     

NEDD1-dependent recruitment of the gamma-tubulin ring complex to the centrosome is necessary for centriole duplication and spindle assembly

The centrosome is the major microtubule organizing structure in somatic cells. Centrosomal microtubule nucleation depends on the protein gamma-tubulin. In mammals, gamma-tubulin associates with additional proteins into a large complex, the gamma-tubulin ring complex (gammaTuRC). We characterize NEDD1, a centrosomal protein that associates with gammaTuRCs. We show that the majority of gammaTuRCs assemble even after NEDD1 depletion but require NEDD1 for centrosomal targeting. In contrast, NEDD1 can target to the centrosome in the absence of gamma-tubulin. NEDD1-depleted cells show defects in centrosomal microtubule nucleation and form aberrant mitotic spindles with poorly separated poles. Similar spindle defects are obtained by overexpression of a fusion protein of GFP tagged to the carboxy-terminal half of NEDD1, which mediates binding to gammaTuRCs. Further, we show that depletion of NEDD1 inhibits centriole duplication, as does depletion of gamma-tubulin. Our data suggest that centriole duplication requires NEDD1-dependent recruitment of gamma-tubulin to the centrosome.     

Alterations in the composition of the supramucosal defense barrier in relation to disease severity of ulcerative colitis.

Mucin glycoproteins and trefoil peptides play an important role in protection and repair of the gastrointestinal epithelium. This study investigates alterations in mucin and trefoil peptide gene expression and product localization in ulcerative colitis (UC). Product localization and message expression of mucin MUC1 to 6 and trefoil peptide TFF1 to 3 genes was analyzed in rectosigmoid tissue from a cohort of patients with active UC and compared with that of normal colorectal mucosa. MUC1 expression was upregulated in severe UC at the site of rupture of crypt abscesses. Reduction in MUC2 expression occurred in UC adjacent to ulceration. No alteration in MUC3 or MUC4 gene expression was detectable in UC compared with normal colorectal mucosa. No ectopic expression of MUC5AC, MUC5B, or MUC6 was identified in UC. Ectopic TFF1 expression was identified in tissues eliciting histological features of severe disease. Decreased TFF3 localization was demonstrated in UC tissues, but no TFF2 expression was detected in any colorectal specimens. Subtle alterations in composition of the supramucosal defense barrier exist in UC and vary in relation to clinical severity of disease. There is upregulation in mucin MUC1 at crypt abscesses and neo-expression of TFF1 trefoil peptide in severe disease.     

Metabolic changes associated with active water vapour absorption in the mealworm Tenebrio molitor L. (Coleoptera, Tenebrionidae): a microcalorimetric study

Water vapour absorption (WVA) is an important mechanism for water gain in several xeric insects. Theoretical calculations indicate that the energetic cost of WVA should be small (5-10% of standard metabolic rate) assuming realistic efficiencies. In this study we explored the relationship between WVA, metabolic heat flux (HFmet.) and CO2 release in larvae of Tenebrio molitor using microcalorimetry. By comparing metabolic heat flux with the catabolic rate estimated from VCO2 , we were able to differentiate anabolic and catabolic rates prior to and during WVA, while simultaneously monitoring water exchange. Three to four hours before the onset of WVA, larvae showed clear increases in HFmet. and catabolic flux, and a simultaneous decrease in anabolic flux. Following the onset of WVA, HFmet. decreased again until indistinguishable from control (non-absorbing) values. Possible factors contributing to the "preparatory phase" are discussed, including mobilization of Malpighian tubule transporters and muscular activity in the rectum. Absorbing larvae reduced the water activity of the calorimetric cell to 0.906, agreeing with gravimetric estimates of the critical equilibrium activity. Periods of movement during WVA coincided with decreased uptake fluxes, consistent with the animal's hydrostatic skeleton and the need to close the anus to generate pressure increases in the haemocoel.