Generators for the SIS/DIS region

We describe how the main neutrino interaction generators (GENIE, NEUT and NuWro) used by current neutrino oscillation experiments treat the shallow and deep inelastic region. We then compare their predictions for charged current events in this region, in terms of transferred momentum as well as multiplicities for different types of hadrons. We present additional comparisons in the low hadronic invariant mass region, where the generators use different custom models.Comment: 8 pages, 8 figures. Proceedings for a talk presented at NuINT201

The Total Artificial Heart and the Dilemma of Deactivation

It is widely believed to be permissible for a physician to discontinue any treatment upon the request of a competent patient. Many also believe it is never permissible for a physician to intentionally kill a patient. I argue that the prospect of deactivating a patient’s artificial heart presents us with a dilemma: either the first belief just mentioned is false or the second one is. Whichever horn of the dilemma we choose has significant implications for contemporary medical ethics

On the trail of the 'new head' in Les Treilles

The vertebrate brain develops in association with neighboring tissues: neural crest, placodes, mesoderm and endoderm. The molecular and evolutionary relationships between the forming nervous system and the other craniofacial structures were at the focus of a recent meeting at the Fondation des Treilles in France. Entitled 'Relationships between Craniofacial and Neural Development', the meeting brought together researchers working on diverse species, the findings of whom provide clues as to the origin and diversity of the brain and facial regions that are involved in forming the 'new head' of vertebrates

From egg to organism

The embryo is a remarkable self-assembly machine. From a single cell, the fertilized egg, arises all of the differentiated cell types of the body. Embryos unfold in an elegantly choreographed manner that we strive to understand by observing the process, dissecting it into smaller bits, and mucking up the works by expressing too much or too little of some protein. Yet the mystery remains and, as knowledge and technology advance, we understand more about the depth of its complexity than about the process itself

Gene regulatory network underlying neural crest formation

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The CLSTM system: reducing settlement risk in foreign exchange transactions.

The launch of the CLSTM system on 9 September 2002 marked the completion of an ambitious project undertaken by the banking sector following the G10 central banks’ recommendations on reducing settlement risk in foreign exchange transactions. The CLS system is owned by 66 of the largest foreign exchange-dealing banks, including 4 French banks. In the first phase, 7 currencies (euro, US dollar, sterling, yen, Swiss franc, Canadian dollar and Australian dollar) will be eligible for CLS. The system is bound to establish itself as the standard “market infrastructure” for settling foreign exchange transactions. The first section of this article looks at the CLS system in light of the central banks’ joint efforts with the banking industry to reduce settlement risk in foreign exchange transactions. The second section describes the CLS operating principles and its contribution to controlling settlement risk. The third section discusses the central banks’ role in the oversight of the CLS project. The final section looks at the impact that the implementation of the system may have on payment activities.

Relaxation Dynamics of Photoexcited Charge Carriers at the Bi(111) Surface

Bi possesses intriguing properties due to its large spin-orbit coupling, e.g. as a constituent of topological insulators. While its electronic structure and the dynamics of electron-phonon coupling have been studied in the past, photo-induced charge carriers have not been observed in the early phases of their respective relaxation pathways. Using two-photon photoemission (2PPE) we follow the de-excitation pathway of electrons along the unoccupied band structure and into a bulk hole pocket. Two decay channels are found, one of which involves an Auger process. In the hole pocket, the electrons undergo an energetic stabilization and recombine with the corresponding holes with an inverse rate of 2.5~ps. Our results contribute to the understanding of the charge carrier relaxation processes immediately upon photo-excitation, particularly along the $\Gamma T$-line where the electron dynamics have not been probed with time-resolved 2PPE so far.Comment: 8 pages, 5 figure

Unoccupied electronic band structure of the semi-metallic Bi(111) surface probed with two-photon photoemission

While many photoemission studies have dealt with both the bulk band structure and various surface states and resonances, the unoccupied electronic structure above the Fermi level of the Bi(111) surface has not yet been measured directly although understanding of this model semi-metal is of great interest for topological insulators, spintronics and related fields. We use angle-resolved two-photon photoemission to directly investigate the occupied and unoccupied p bands of Bi, including the bulk hole pocket at the T point, as well as the image potential states and surface states of Bi(111).Comment: 9 pages, 7 figure

A novel spalt gene expressed in branchial arches affects the ability of cranial neural crest cells to populate sensory ganglia

Cranial neural crest cells differentiate into diverse derivatives including neurons and glia of the cranial ganglia, and cartilage and bone of the facial skeleton. Here, we explore the function of a novel transcription factor of the spalt family that might be involved in early cell-lineage decisions of the avian neural crest. The chicken spalt4 gene (csal4) is expressed in the neural tube, migrating neural crest, branchial arches and, transiently, in the cranial ectoderm. Later, it is expressed in the mesectodermal, but not neuronal or glial, derivatives of midbrain and hindbrain neural crest. After over-expression by electroporation into the cranial neural tube and neural crest, we observed a marked redistribution of electroporated neural crest cells in the vicinity of the trigeminal ganglion. In control-electroporated embryos, numerous, labeled neural crest cells ([similar]80% of the population) entered the ganglion, many of which differentiated into neurons. By contrast, few ([similar]30% of the population) spalt-electroporated neural crest cells entered the trigeminal ganglion. Instead, they localized in the mesenchyme around the ganglionic periphery or continued further ventrally to the branchial arches. Interestingly, little or no expression of differentiation markers for neurons or other cell types was observed in spalt-electroporated neural crest cells

Avian neural crest cell attachment to laminin: involvement of divalent cation dependent and independent integrins

The mechanisms of neural crest cell interaction with laminin were explored using a quantitative cell attachment assay. With increasing substratum concentrations, an increasing percentage of neural crest cells adhere to laminin. Cell adhesion at all substratum concentrations was inhibited by the CSAT antibody, which recognizes the chick β_1 subunit of integrin, suggesting that β_(1-)integrins mediate neural crest cell interactions with laminin. The HNK-1 antibody, which recognizes a carbohydrate epitope, inhibited neural crest cell attachment to laminin at low coating concentrations (>1 µg ml^(-1); Low-LM), but not at high coating concentration of laminin (10 µg ml^(-1); High-LM). Attachment to Low-LM occurred in the absence of divalent cations, whereas attachment to High-LM required >0.1 mM Ca^(2+) or Mn^(2+). Neural crest cell adherence to the E8 fragment of laminin, derived from its long arm, was similar to that on intact laminin at high and low coating concentrations, suggesting that this fragment contains the neural crest cell binding site(s). The HNK-1 antibody recognizes a protein of 165,000 Mr which is also found in immunoprecipitates using antibodies against the β_1 subunit of integrin and is likely to be an integrin alpha subunit or an integrin-associated protein. Our results suggest that the HNK-1 epitope on neural crest cells is present on or associated with a novel or differentially glycosylated form of β_(1-)integrin, which recognizes laminin in the apparent absence of divalent cations. We conclude that neural crest cells have at least two functionally independent means of attachment to laminin which are revealed at different substratum concentrations and/or conformations of laminin