Second-Hand Stress: Neurobiological Evidence for a Human Alarm Pheromone

Alarm pheromones are airborne chemical signals, released by an individual into the environment, which transmit warning of danger to conspecifics via olfaction. Using fMRI, we provide the first neurobiological evidence for a human alarm pheromone. Individuals showed activation of the amygdala in response to sweat produced by others during emotional stress, with exercise sweat as a control; behavioral data suggest facilitated evaluation of ambiguous threat

The “Data Visualization Clinic”: a library-led critique workshop for data visualization

Background: The authors’ main university library and affiliated academic medical center library sought to increase library programming around data visualization, a new service area for both libraries. Additionally, our institution is home to many researchers with a strong interest in data visualization but who are generally working in isolation of one another. Case Presentation: This case study describes an innovative workshop, the “Data Visualization Clinic,” where members of our library’s community bring in data visualization projects such as figures in papers, projects hosted online, and handouts and receive constructive feedback from a group of peers. The authors detail the process of hosting a clinic and the feedback that we received from participants. Conclusions: The “Data Visualization Clinic” offers a viable workshop to leverage expertise of library users and build the library’s reputation as a hub of data visualization services without heavy investment in infrastructure like special monitors or coding skills. That said, it faces the challenge of relying on the participation of the broader community, which is often pressed for time. The event can also serve as an opportunity for researchers who have an interest in data visualization to meet and network

Ruptured abdominal aortic aneurysm, a “two-hit” ischemia/reperfusion injury: Evidence from an analysis of oxidative products

AbstractPurpose: Ruptured abdominal aortic aneurysm (RAAA) remains a lethal condition despite improvements in perioperative care. The consequences of RAAA are hypothesized to result from a combination of two ischemia/reperfusion events: hemorrhagic shock and lower torso ischemia. Ischemia/reperfusion results in tissue injury by diverse mechanisms, which include oxygen free radical–mediated injury produced from activated neutrophils, xanthine oxidase, and mitochondria. Oxygen-free radicals attack membrane lipids, resulting in membrane and subsequently cellular dysfunction that contributes to postoperative organ injury/failure. The purpose of this investigation was to quantify the oxidative injury that occurs as a result of the ischemia/reperfusion events in RAAAs and elective AAAs. Methods: Blood samples were taken from 22 patients for elective AAA repair and from 14 patients for RAAA repair during the perioperative period. Plasma F2 -isoprostanes were extracted, purified, and measured with an enzyme immunoassay. Aldehydes and acyloins were purified and quantified. Neutrophil oxidative burst was measured in response to a receptor independent stimulus (phorbol 12-myristate 13-acetate) with luminol-based chemiluminescence. Results: Plasma from patients with RAAAs showed significantly elevated F2 -isoprostane levels on arrival at hospital and were significantly elevated as compared with the levels of patients for elective repair throughout the perioperative period (two-way analysis of variance, P < .0001). Multiple regression showed a significant relationship between the phagocyte oxidative activity and F2 -isoprostane levels (P < .013). Total acyloin levels were significantly higher in patients with RAAAs as compared with the levels in elective cases. Conclusion: The F2 -isoprostane levels, specific markers of lipid peroxidation, showed that patients with RAAAs had two phases of oxidative injury: before arrival at hospital and after surgery. The significant relationship between the postoperative increases in F2 -isoprostane levels and the neutrophil oxidant production implicates neutrophils in the oxidative injury that occurs after RAAA. New therapeutic interventions that attenuate neutrophil-mediated oxidant injury during reperfusion may decrease organ failure and ultimately mortality in patients with RAAAs. (J Vasc Surg 1999;30:219-28.

Sok: Security and privacy in implantable medical devices and body area networks.

Abstract-Balancing security, privacy, safety, and utility is a necessity in the health care domain, in which implantable medical devices (IMDs) and body area networks (BANs) have made it possible to continuously and automatically manage and treat a number of health conditions. In this work, we survey publications aimed at improving security and privacy in IMDs and health-related BANs, providing clear definitions and a comprehensive overview of the problem space. We analyze common themes, categorize relevant results, and identify trends and directions for future research. We present a visual illustration of this analysis that shows the progression of IMD/BAN research and highlights emerging threats. We identify three broad research categories aimed at ensuring the security and privacy of the telemetry interface, software, and sensor interface layers and discuss challenges researchers face with respect to ensuring reproducibility of results. We find that while the security of the telemetry interface has received much attention in academia, the threat of software exploitation and the sensor interface layer deserve further attention. In addition, we observe that while the use of physiological values as a source of entropy for cryptographic keys holds some promise, a more rigorous assessment of the security and practicality of these schemes is required

Tranilast inhibits hormone refractory prostate cancer cell proliferation and suppresses transforming growth factor Β1-associated osteoblastic changes

BACKGROUND Tranilast is a therapeutic agent used in treatment of allergic diseases, although it has been reported to show anti-tumor effects on some cancer cells. To elucidate the effects of tranilast on prostate cancer, we investigated the mechanisms of its anti-tumor effect on prostate cancer. METHODS The anti-tumor effects and related mechanisms of tranilast were investigated both in vitro on prostate cancer cell lines and bone-derived stromal cells, and in vivo on severe combined immunodeficient (SCID) mice. We verified its clinical effect in patients with advanced hormone refractory prostate cancer (HRPC). RESULTS Tranilast inhibited the proliferation of LNCaP, LNCaP-SF, and PC-3 cells in a dose-dependent manner and growth of the tumor formed by inoculation of LNCaP-SF in the dorsal subcutis and in the tibia of castrated SCID mice. Flow cytometry and TUNEL assay revealed induction of cell cycle arrest and apoptosis by tranilast. Tranilast increased expression of proteins involved in induction of cell cycle arrest and apoptosis. Coculture with bone-derived stromal cells induced proliferation of LNCaP-SF cells. Tranilast also suppressed secretion of transforming growth factor Β1 (TGF-Β1) from bone-derived stromal cells, which induced their differentiation. Moreover, tranilast inhibited TGF-Β1-mediated differentiation of bone-derived stromal cells and LNCaP-SF cell migration induced by osteopontin. In the clinical investigation, PSA progression was inhibited in 4 of 16 patients with advanced HRPC. CONCLUSIONS These observations suggest that tranilast may be a useful therapeutic agent for treatment of HRPC via the direct inhibitory effect on cancer cells and suppression of TGF-Β1-associated osteoblastic changes in bone metastasis. Prostate 69:1222–1234, 2009. © 2009 Wiley-Liss, Inc.Peer Reviewedhttp://deepblue.lib.umich.edu/bitstream/2027.42/63038/1/20975_ftp.pd

Desenvolvimento embrionário in vitro de oócitos bovinos mantidos em líquido folicular ou TCM-hepes

In order to evaluate the effect of a transport medium on the rate of in vitro embryonic development, 1381 Cumulus-oocyte Complexes (COC) were obtained by aspiration of 2-8mm diameter follicles witch were randomly divided in 4 treatment groups. The Control group was formed by oocytes matured in modified TCM-199 for 24h, incubated at 39°C and 5,00% CO2 with saturated humidity. The group 1 (WB24h), included oocytes matured in 1.0mL tubes containing TCM-HEPES (5.95mg/mL), in water bath (WB) at 39°C for 24h. The group 2 (FFb6C18h), included oocytes kept in bovine follicular fluid (FFb) for 6h at 30°C followed by a period of 18h maturation under the same conditions as the Control group and with the oocytes maintained in FFb followed by 18h IVM under the same conditions as the group 1, group 3 (FFb6WB18h). Fertilization was performed in FERT-TALP for 18h. Zygotes were cultured in SOFaaci under mineral oil within gasified bags. The cleavage rate differed (P&lt;0.05) between the Control and FFb6BM18h groups. However, there was no difference on the D7 and D9 blastocyst rates and on the percentage of blastocyst ecloded. It was concluded that it is possible to maintain the oocytes in FFb for 6h at 30°C before 18h IVM, or to proote the transport and maturation of the oocytes for 24h, in TCM-HEPES and water-bath at 39°C, without compromising embryonic development. The simplification of MIV showed in this experiment through of tubes (1.0mL) replete with TCM-HEPES and holding in water bath at 39°C, could be a viable and practice for the bovine programs of OPU/PIV.Complexos Cumulus-Oócito (CCO) bovinos foram divididos em 4 grupos para avaliar o seu comportamento durante a manutenção em LFb e maturação in vitro (MIV) em TCM-199 com ou sem Hepes. CCO MIV por 24h em TCM-199 em estufa a 39°C com 5,00% de CO2 (Controle) tiveram o seu desenvolvimento comparado ao de CCO MIV em tubos repletos de TCM-HEPES (5,95 mg/mL), em banho-maria (BM) a 39ºC por 24h (Grupo 1 - BM24h), ao de CCO mantidos em líquido folicular bovino (LFb), por 6h a 30ºC seguido de maturação por 18h nas mesmas condições que o grupo Controle (Grupo 2 - LFb6C18h) e ao de CCO mantidos em LFb seguido da maturação por 18h sob as mesmas condições que o grupo 1 (Grupo 3 - LFb6BM18h). A fecundação foi realizada em FERT-TALP por 18h. Os zigotos foram cultivados em SOFaaci, sob óleo mineral, em bolsas plásticas gaseificadas. A taxa de clivagem no Grupo Controle foi superior a do Grupo 3 (P&lt;0,05), mas não houve diferença no percentual de blastocistos no D7 e D9 e no de blastocistos eclodidos entre os 4 grupos. Portanto, oócitos podem ser mantidos por 6h em LFb, a 30ºC, antes da maturação em TCM-HEPES por 18h ou ser maturados por 24h, em TCM-HEPES, em banho-maria a 39ºC, sem atmosfera gasosa controlada. A simplificação da MIV aqui introduzida através do preenchimento de tubos de 1,0mL com TCM-HEPES e manutenção em banho-maria a 39ºC, poderá ser uma opção viável e prática para os programas de OPU/PIV em bovinos

Lack of group X secreted phospholipase A₂ increases survival following pandemic H1N1 influenza infection

The role of Group X secreted phospholipase A2 (GX-sPLA2) during influenza infection has not been previously investigated. We examined the role of GX-sPLA2 during H1N1 pandemic influenza infection in a GX-sPLA2 gene targeted mouse (GX−/−) model and found that survival after infection was significantly greater in GX−/− mice than in GX+/+ mice. Downstream products of GX-sPLA2 activity, PGD2, PGE2, LTB4, cysteinyl leukotrienes and Lipoxin A4 were significantly lower in GX−/− mice BAL fluid. Lung microarray analysis identified an earlier and more robust induction of T and B cell associated genes in GX−/− mice. Based on the central role of sPLA2 enzymes as key initiators of inflammatory processes, we propose that activation of GX-sPLA2 during H1N1pdm infection is an early step of pulmonary inflammation and its inhibition increases adaptive immunity and improves survival. Our findings suggest that GX-sPLA2 may be a potential therapeutic target during influenza

Duchamp's Erotic Stereoscopic Exercises

This article explores certain links between medicine and art, with regard to their use of stereoscopy. I highlight a work by the artist Marcel Duchamp (the ready-made Stéréoscopie a la Main) and stereoscopic cards used in ophthalmic medicine. Both instances involve the drawing of graphic marks over previously existing stereoscopic cards. This similarity between Stéréoscopie a la Main and stereoscopic cards is echoed in the form of "stereoscopic exercises." Stereoscopic exercises were prescribed by doctors to be performed with the stereoscope as early as 1864. Stereoscopic cards were widely diffused in the 19th century, often promoted as "stay-at-home travel." It was over such kinds of materials that both Marcel Duchamp and doctors of ophthalmic medicine drew their graphic marks. I explore Duchamp's Stéréoscopie a la Main as a hypothetical basis for stereoscopic exercises of different types, proposing that this rectified ready-made is the locus for erotic stereoscopic exercises.Este artigo busca explorar certos elos entre a medicina e a arte por meio da estereoscopia. Destaca-se uma obra do artista Marcel Duchamp (o ready-made Stéréoscopie a la Main) e cartões estereoscópicos usados na oftalmologia. As duas instâncias envolvem o desenho de marcas gráficas sobre cartões estereoscópicos pré-existentes. A similaridade entre Stéréoscopie a la Main e os ditos cartões ecoa também na forma dos exercícios estereoscópicos. O cartão estereoscópico foi amplamente difundido na segunda metade do séc. XIX, frequentemente na forma da "viagem sem sair de casa." Foi sobre esse tipo de material que tanto médicos quanto Marcel Duchamp desenharam suas marcas. Explora-se a obra Stéréoscopie a la Main como um sítio hipotético para uma espécie de exercício, propondo que tal ready-made retificado seja um lugar para exercícios estereoscópicos eróticos

Desenvolvimento embrionário de oócitos bovinos mantidos em fluido folicular bovino de folículos de diferentes diâmetros

Bovine oocytes have been maintained in the follicular fluid to be transported and to increase their competence, before maturation. Eight hundred eighty-one (881) oocytes, aspirated from bovine slaughterhouse ovaries, were used to evaluate the effect of holding bovine oocytes in follicular fluid (FF) of bovine follicles of different diameters on the rate of embryo development. The oocytes were randomly distributed in four treatments with seven replicates each: The control group (n=217) was constituted by oocytes matured for 24h in modified TCM-199 with Estrus Mare Serum (EMS), pyruvate and rFSH-h in incubator with 5,00% CO2, 39°C and saturated humidity. In the FFsmall group (3 to 5mm follicles; n=216), the oocytes were held for 6h in follicular fluid at 30°C and matured for 18h in the same conditions of the Control-group. The oocytes of the FFmedium group (5,1-8mm follicles; n=226) and of the FFlarge group (&gt;;8,1mm follicles; n=222) were held in follicular fluid and matured like FFsmall. Fertilization was accomplished during 18h and, after this, the zygotes were cultured for 8 days in SOFaaci medium + 5,00% EMS in incubator at 39°C using plastic bags gasified with 5,00%CO2, 5,00%O2 and 90,00%N2. FFsmall oocytes produced a lower (P;0,05) between the groups. Follicular fluid of medium and large follicles could be used to hold for 6h at 30°C bovine oocytes before their maturation for 18h.Oócitos bovinos têm sido mantidos em fluido folicular como meio para transporte e para aumento de sua competência, antes da maturação. Oitocentos e oitenta e um (881) oócitos foram aspirados de folículos de 2 a 8mm, de ovários de abatedouro, para avaliar o efeito da manutenção de oócitos bovinos em fluido folicular bovino de folículos de diferentes tamanhos sobre o desenvolvimento embrionário. Os oócitos foram distribuídos aleatoriamente em quatro tratamentos, com sete repetições cada. No grupo controle (n=217), os oócitos foram maturados por 24h em TCM-199 com Soro de Égua em Estro (SEE), piruvato e rFSH-h, em estufa a 39°C, com 5,00% de CO2 e umidade saturada. No tratamento FFpequeno (n=216), os oócitos foram mantidos por 6h em fluido folicular de folículos de 3 a 5mm a 30°C e posteriormente maturados por 18h nas mesmas condições do grupo controle. Os oócitos dos tratamentos FFmédio (n=226) e FFgrande (n=222) foram mantidos em fluido folicular de folículos com 5,1 a 8mm e folículos maiores de 8,1mm, respectivamente e, após, maturados por 18h. Após a fecundação por 18h, os zigotos foram cultivados por 8 dias em SOFaaci com 5,00% de SEE, em estufa a 39°C, em bolsas gaseificadas com 5,00%CO2, 5,00%O2 e 90,00%N2. Oócitos do grupo FFpequeno resultaram em menor (P;0,05) entre os grupos. O fluido folicular de folículos médios e grandes pode ser utilizado para o manutenção de oócitos bovinos por 6h a 30°C, antes da maturação por 18h