Technological Analysis of the World’s Earliest Shamanic Costume: A Multi-Scalar,Experimental Study of a Red Deer Headdress from the Early Holocene Site of Star Carr,North Yorkshire,UK

Shamanic belief systems represent the first form of religious practice visible within the global archaeological record. Here we report on the earliest known evidence of shamanic costume: modified red deer crania headdresses from the Early Holocene site of Star Carr (c. 11 kya). More than 90% of the examples from prehistoric Europe come from this one site, establishing it as a place of outstanding shamanistic/cosmological significance. Our work, involving a programme of experimental replication, analysis of macroscopic traces, organic residue analysis and 3D image acquisition, metrology and visualisation, represents the first attempt to understand the manufacturing processes used to create these artefacts. The results produced were unexpected—rather than being carefully crafted objects, elements of their production can only be described as expedient.     

Mapping quantitative trait loci for heat tolerance of reproductive traits in tomato (<Emphasis Type="Italic">Solanum lycopersicum</Emphasis>)

Global warming has become a worldwide concern due to its adverse effects on agricultural output. In particular, long-term mildly high temperatures interfere with sexual reproduction and thus fruit and seed set. To uncover the genetic basis of observed variation in tolerance against heat, a bi-parental F₂ mapping population from two contrasting cultivars, i.e. Nagcarlang and NCHS-1, was generated and phenotyped under continuous mild heat conditions for a number of traits underlying reproductive success, i.e. pollen viability, pollen number, style length, anther length, style protrusion, female fertility and flowering characteristics, i.e. inflorescence number and flowers per inflorescence. Quantitative trait loci (QTLs) were identified for most of these traits, including a single, highly significant one for pollen viability, which accounted for 36% of phenotypic variation in the population and modified pollen viability under high temperature with around 20%. QTLs for some traits colocalised, indicating trait dependency or pleiotropic-effect loci. We conclude that a limited set of major genes determines differences in performance of reproductive traits under continuous mild heat in tomato. The results contribute to our fundamental understanding of pollen thermotolerance and may support development of more heat-tolerant tomato varieties.     

The relationship between gap formation and grip-to-grip displacement during cyclic testing of repaired flexor tendons

The assessment of repair site gap formation during cyclic loading of reconstructed flexor tendons provides important data on the performance of repair techniques in the early postoperative period. This study describes our cyclic testing protocol and evaluates the relationship between changes in optical gap and grip-to-grip displacement. Sixteen sheep hind limb deep flexor tendons were randomized into four repair groups (n=4 per group): a 2-strand repair (modified Kessler) and 4-strand repair (Adelaide), both with and without a simple running peripheral suture. Repaired tendons were cycled for 1000 cycles at appropriate rehabilitation loads for the reconstruction. Tendons were paused at 18 pre-determined cycle points to measure gap and displacement. A strong positively linear relationship between gap and displacement was demonstrated for all repair groups (R²>0.90). An initial non-linear region during the first 10 cycles was noted with some combined core and peripheral repairs. Although trends in displacement after 10 cycles can be used to reflect gapping behaviour, direct optical measurement of gap remains preferable. We hypothesized that the adjustment of suture strands and equilibration of forces within the reconstruction occurs mostly during the initial 10 cycles. Gap–cycle curves provide a good illustration of dynamic changes at the repair site, and should be added more frequently to cyclic testing studies.     

Adjusting for selection bias in retrospective, case-control studies

Retrospective case–control studies are more susceptibleto selection bias than other epidemiologic studies as by designthey require that both cases and controls are representativeof the same population. However, as cases and control recruitmentprocesses are often different, it is not always obvious thatthe necessary exchangeability conditions hold. Selection biastypically arises when the selection criteria are associatedwith the risk factor under investigation. We develop a methodwhich produces bias-adjusted estimates for the odds ratio. Ourmethod hinges on 2 conditions. The first is that a variablethat separates the risk factor from the selection criteria canbe identified. This is termed the "bias breaking" variable.The second condition is that data can be found such that a bias-correctedestimate of the distribution of the bias breaking variable canbe obtained. We show by means of a set of examples that suchbias breaking variables are not uncommon in epidemiologic settings.We demonstrate using simulations that the estimates of the oddsratios produced by our method are consistently closer to thetrue odds ratio than standard odds ratio estimates using logisticregression. Further, by applying it to a case–controlstudy, we show that our method can help to determine whetherselection bias is present and thus confirm the validity of studyconclusions when no evidence of selection bias can be found.     

Development of pyrF-Based Genetic System for Targeted Gene Deletion in Clostridium thermocellum and Creation of a pta Mutant

We report development of a genetic system for making targeted gene knockouts in Clostridium thermocellum, a thermophilic anaerobic bacterium that rapidly solubilizes cellulose. A toxic uracil analog, 5-fluoroorotic acid (5-FOA), was used to select for deletion of the pyrF gene. The ΔpyrF strain is a uracil auxotroph that could be restored to a prototroph via ectopic expression of pyrF from a plasmid, providing a positive genetic selection. Furthermore, 5-FOA was used to select against plasmid-expressed pyrF, creating a negative selection for plasmid loss. This technology was used to delete a gene involved in organic acid production, namely pta, which encodes the enzyme phosphotransacetylase. The C. thermocellum Δpta strain did not produce acetate. These results are the first examples of targeted homologous recombination and metabolic engineering in C. thermocellum, a microbe that holds an exciting and promising future in the biofuel industry and development of sustainable energy resources.Conversion of cellulosic biomass using saccharolytic fermentative microorganisms without the addition of purified cellulase and hemicellulase enzymes is a promising approach for low-cost production of renewable fuels and chemicals (22, 23). Thermophilic, cellulolytic bacteria are one departure point for development of microorganisms with the requisite capabilities for such consolidated bioprocessing (CBP), with Clostridium thermocellum being exemplary in this regard. As reviewed elsewhere (6, 22), C. thermocellum is a Gram-positive organism able to ferment cellulose and products of cellulose solubilization to ethanol, acetic acid, lactic acid, formic acid, hydrogen, and CO₂. C. thermocellum appears to be a cellulose-utilizing specialist (6, 8) and produces a multienzyme cellulose-solubilizing complex termed a cellulosome (2, 3, 9).Metabolic engineering is required in order to increase the yield of ethanol or other desired products from mixed-product fermentation, such as that carried out by Clostridium thermocellum. Comprehensive work directed to this end has been carried out with genetically tractable organisms, such as Escherichia coli, resulting in high or near-theoretical yields achieved for ethanol (35, 36), other native products (21, 25), and nonnative products (7, 12). In these organisms, genetic systems involving both positive and negative selection markers have been employed in order to facilitate reuse of the same marker and to develop marker-free strains. One prominent system in the category involves use of the gene encoding the enzyme orotidine 5-phosphate decarboxylase (PyrF) (4, 11, 20, 27-29, 39). PyrF participates in de novo pyrimidine biosynthesis but is also a target for the antimetabolite 5-fluoroorotic acid (5-FOA) (4). Thus, cells lacking pyrF are uracil auxotrophs and resistant to 5-FOA, creating an opportunity whereby ectopic expression of pyrF can be selected or counterselected (4).Reliable genetic tractability has been elusive for Clostridium species. Prior to this report, the only Clostridia species in which gene deletion via homologous recombination has been demonstrated are Clostridium acetobutylicum, Clostridium perfringens, and Clostridium septicum. In the first organism, the use of a replicating plasmid for transformation followed by selection and screening for plasmid segregation resulted in a single clone that when analyzed contained a disruption in the gene of interest but not by the expected recombination events (13). The last two organisms have either an unusually high transformation frequency or feasibility for acquiring DNA from E. coli via conjugation, allowing the use of suicide plasmids (1, 16, 19). By comparison, the recently reported method of C. thermocellum transformation consists of a complex and cumbersome electroporation protocol using a custom pulse delivery system (37, 38). In our hands, efficiency of the C. thermocellum electrotransformation system does not compare with that of typical model organisms and does not enable the use of nonreplicating plasmids as a means of gene manipulation. Alternatively, group II intron technology has been used to inactivate gene targets in clostridia that were previously characterized as genetically intractable, but systems described to date have a temperature restriction that make such approaches incompatible with thermophilic clostridia (14, 15, 34).The only C. thermocellum mutant characterized genetically was isolated following a random mutagenesis and enrichment for cells that did not adhere to cellulose (43). The random mutagenesis approach is limited, in the sense that it does not lend itself well to reverse genetics, as many desired mutations lack selectable or screenable phenotypes. For instance, attempts have been made, with little success, to isolate saccharolytic thermophiles containing lesions in the pta-ack operon responsible for acetate production by selective enrichment using antimetabolites (26). In contrast, the creation of a Thermoanaerobacterium saccharolyticum Δpta-ack strain has been achieved using selectable markers that serve as a proxy for the events leading to targeted gene deletion (32). Motivated by the potential of microbial cellulose processing and the attributes of C. thermocellum, we undertook to develop a gene deletion system based on the pyrF gene.     

Saccharomyces cerevisiae-Based Molecular Tool Kit for Manipulation of Genes from Gram-Negative Bacteria

A tool kit of vectors was designed to manipulate and express genes from a wide range of gram-negative species by using in vivo recombination. Saccharomyces cerevisiae can use its native recombination proteins to combine several amplicons in a single transformation step with high efficiency. We show that this technology is particularly useful for vector design. Shuttle, suicide, and expression vectors useful in a diverse group of bacteria are described and utilized. This report describes the use of these vectors to mutate clpX and clpP of the opportunistic pathogen Pseudomonas aeruginosa and to explore their roles in biofilm formation and surface motility. Complementation of the rhamnolipid biosynthetic gene rhlB is also described. Expression vectors are used for controlled expression of genes in two pseudomonad species. To demonstrate the facility of building complicated constructs with this technique, the recombination of four PCR-generated amplicons in a single step at >80% efficiency into one of these vectors is shown. These tools can be used for genetic studies of pseudomonads and many other gram-negative bacteria.     

Activation of the selenoprotein SEPS1 gene expression by pro-inflammatory cytokines in HepG2 cells

SEPS1 (also called selenoprotein S, SelS) plays an important role in the production of inflammatory cytokines and its expression is activated by endoplasmic reticulum (ER) stress. In this report, we have identified two binding sites for the nuclear factor kappa B in the human SEPS1 promoter. SEPS1 gene expression, protein levels and promoter activity were all increased 2-3-fold by TNF-alpha and IL-1beta in HepG2 cells. We have also confirmed that the previously proposed ER stress response element GGATTTCTCCCCCGCCACG in the SEPS1 proximate promoter is fully functional and responsive to ER stress. However, concurrent treatment of HepG2 cells with IL-1beta and ER stress produced no additive effect on SEPS1 gene expression. We conclude that SEPS1 is a new target gene of NF-kappaB. Together with our previous findings that SEPS1 may regulate cytokine production in macrophage cells, we propose a regulatory loop between cytokines and SEPS1 that plays a key role in control of the inflammatory response.     

Genome wide gene-expression analysis of facultative reproductive diapause in the two-spotted spider mite Tetranychus urticae

Background

Diapause or developmental arrest, is one of the major adaptations that allows mites and insects to survive unfavorable conditions. Diapause evokes a number of physiological, morphological and molecular modifications. In general, diapause is characterized by a suppression of the metabolism, change in behavior, increased stress tolerance and often by the synthesis of cryoprotectants. At the molecular level, diapause is less studied but characterized by a complex and regulated change in gene-expression. The spider mite Tetranychus urticae is a serious polyphagous pest that exhibits a reproductive facultative diapause, which allows it to survive winter conditions. Diapausing mites turn deeply orange in color, stop feeding and do not lay eggs.

Results

We investigated essential physiological processes in diapausing mites by studying genome-wide expression changes, using a custom built microarray. Analysis of this dataset showed that a remarkable number, 11% of the total number of predicted T. urticae genes, were differentially expressed. Gene Ontology analysis revealed that many metabolic pathways were affected in diapausing females. Genes related to digestion and detoxification, cryoprotection, carotenoid synthesis and the organization of the cytoskeleton were profoundly influenced by the state of diapause. Furthermore, we identified and analyzed an unique class of putative antifreeze proteins that were highly upregulated in diapausing females. We also further confirmed the involvement of horizontally transferred carotenoid synthesis genes in diapause and different color morphs of T. urticae.

Conclusions

This study offers the first in-depth analysis of genome-wide gene-expression patterns related to diapause in a member of the Chelicerata, and further adds to our understanding of the overall strategies of diapause in arthropods.

Electronic supplementary material

The online version of this article (doi:10.1186/1471-2164-14-815) contains supplementary material, which is available to authorized users.     

PKCα-Specific Phosphorylation of the Troponin Complex in Human Myocardium: A Functional and Proteomics Analysis

Aims

Protein kinase Cα (PKCα) is one of the predominant PKC isoforms that phosphorylate cardiac troponin. PKCα is implicated in heart failure and serves as a potential therapeutic target, however, the exact consequences for contractile function in human myocardium are unclear. This study aimed to investigate the effects of PKCα phosphorylation of cardiac troponin (cTn) on myofilament function in human failing cardiomyocytes and to resolve the potential targets involved.

Methods and Results

Endogenous cTn from permeabilized cardiomyocytes from patients with end-stage idiopathic dilated cardiomyopathy was exchanged (∼69%) with PKCα-treated recombinant human cTn (cTn (DD+PKCα)). This complex has Ser23/24 on cTnI mutated into aspartic acids (D) to rule out in vitro cross-phosphorylation of the PKA sites by PKCα. Isometric force was measured at various [Ca²⁺] after exchange. The maximal force (F_max) in the cTn (DD+PKCα) group (17.1±1.9 kN/m²) was significantly reduced compared to the cTn (DD) group (26.1±1.9 kN/m²). Exchange of endogenous cTn with cTn (DD+PKCα) increased Ca²⁺-sensitivity of force (pCa₅₀ = 5.59±0.02) compared to cTn (DD) (pCa₅₀ = 5.51±0.02). In contrast, subsequent PKCα treatment of the cells exchanged with cTn (DD+PKCα) reduced pCa₅₀ to 5.45±0.02. Two PKCα-phosphorylated residues were identified with mass spectrometry: Ser198 on cTnI and Ser179 on cTnT, although phosphorylation of Ser198 is very low. Using mass spectrometry based-multiple reaction monitoring, the extent of phosphorylation of the cTnI sites was quantified before and after treatment with PKCα and showed the highest phosphorylation increase on Thr143.

Conclusion

PKCα-mediated phosphorylation of the cTn complex decreases F_max and increases myofilament Ca²⁺-sensitivity, while subsequent treatment with PKCα in situ decreased myofilament Ca²⁺-sensitivity. The known PKC sites as well as two sites which have not been previously linked to PKCα are phosphorylated in human cTn complex treated with PKCα with a high degree of specificity for Thr143.