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Acta Physiologica Hungarica
Authors:
Jeremy Loenneke
,
C. Fahs
,
R. Thiebaud
,
L. Rossow
,
T. Abe
,
Xin Ye
,
D. Kim
, and
M. Bemben

The purpose of this study was to investigate the potential mechanisms behind the blood flow restriction (BFR) stimulus in the absence of exercise. Nine participants completed a 10 minute time control and then a BFR protocol. The protocol was five, 5-minute bouts of inflation with 3-minutes of deflation between each bout. The pressure was set relative to each individual’s thigh circumference. Significant increases in muscle thickness were observed for both the vastus lateralis (VL) [6%, p = 0.027] and rectus femoris (RF) [22%, p = 0.001] along with a significant decrease in plasma volume [15%, p = 0.001]. Ratings of discomfort during the BFR protocol peaked at 2.7 (light discomfort). There were no significant changes with whole blood lactate, electromyography (EMG), or heart rate (HR), however, there was a trend for a significant increase in HR during the 5th inflation (p = 0.057). In conclusion, this is the first study to demonstrate that the attenuation of both muscle atrophy and declines in strength previously observed with brief applications of BFR may have been mediated through an acute fluid shift induced increase in muscle size. This is supported by our finding that the changes in muscle thickness are maintained even after the cuffs have been removed.

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Abstract  

The concentrations and distributions of total halogen (TX), extractable organohalogen (EOX) and extractable persistent organohalogen (EPOX) were determined in 20 kinds of yogurt specimens collected from Chinese supermarkets using neutron activation analysis (NAA) and gas chromatography equipped with a 63Ni electron capture detector (GC-ECD). The results indicated that the halogens in yogurt mainly existed as non-extractable organohalogen compounds. About 25–30% of EOX was EPOX. EOCl and EPOCl were the main organohalogen species in yogurt. The average concentration of the identified organochlorine, such as organochlorine pesticides (OCPs) and polychlorinated biphenyls (PCBs), was below 4% of EPOCl.

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The present study was to evaluate the survival rate of free and encapsulated Bifidobacterium bifidum BB28 under simulated gastrointestinal conditions and its stability during storage. Results showed that non-microencapsulated Bifidobacterium bifidum BB28 was more susceptible to simulated gastrointestinal conditions than microencapsulated bacteria. Microencapsulated Bifidobacterium BB28 exhibited a lower population reduction than free cells during exposure to simulated gastrointestinal conditions, the viable count of monolayer microcapsules, double layer microcapsules, and triple layer microcapsules decreased by nine magnitudes, four magnitudes, and one magnitude after 2 h, respectively. The enteric test showed that the microorganism cells were released from the monolayer, double layer, and triple layer microcapsules completely in 40 min. Moreover, the optimum storage times of free Bifidobacterium BB28, monolayer microcapsules, double layer microcapsules, and triple layer microcapsules were 21 days, 21 days, 28 days, and more than 35 days in orange juice, pure milk, and nutrition Express (a commercially available milk based drink), and the viable counts were maintained at 1×106 CFU g−1 or more, which means that the double layer and triple layer of microcapsules of B. bifidum BB28 have great potential in food application.

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Stripe rust, caused by Puccinia striiformis f. sp. tritici (PST), is one of the most serious diseases of wheat ( Triticum aestivum L.) worldwide. Of 94 Triticum durum/Aegilops tauschii synthetic wheat accessions tested, CI142 (Garza/Boy// Ae. squarrosa 271) was found to be resistant to 6 Chinese PST races. The resistance to stripe rust in CI142 was proven to be controlled by a single dominant gene, tentatively designated YrC142 . Gene postulation showed that the pathogenic specificity of CI142 is different from 21 other lines possessing known resistance genes, such as Yr10, Yr15, Yr24 , and Yr26 , located on chromosome 1B. Bulked segregant analysis (BSA) and F 2 segregation analysis of the CI142/Mingxian 169 cross were used to analyse the SSR markers linked to YrC142 . Five SSR markers were found to be closely associated with YrC142 in the order Xwmc419-YrC142-Xgwm273, Xbarc187-Xgwm18-Xwmc626 , in which the relative genetic distances of these SSR loci to the gene YrC142 were 5.4, 0.8, 0.8, 1.0, and 2.4 cM, respectively. Two SSR markers ( Xgwm273 −162 and Xgwm18 −168 ) distinguished YrC142 from Yr10, Yr15, Yr24 , and Yr26 , suggesting that these 2 SSR markers may be used as diagnostic ones for the gene in a wheat breeding program against stripe rust. Based on these findings, YrC142 is most likely a new gene or a new allele at the Yr26 locus, which provides an opportunity to diversify stripe rust-resistant resources for wheat breeding programs.

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The common wheat line, YW243, developed in our research group, was tested for the resistances of barley yellow dwarf virus (BYDV), powdery mildew (Pm) and stripe rust in field, and was analyzed by molecular markers for convenient trace of the resistant genes in breeding. Genomic in situ hybridization (GISH) analysis and sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) assay further demonstrated that YW243 was a homozygous multiple translocation line of Triticum aestivum, Thinopyrum intermedium and Secale cereale (T7DS·7DL-7XL & 1BL·1RS). The disease resistance test and marker analysis showed that YW243 carried seven resistance genes to the three diseases, including Bdv2 to BYDV on 7DL-7XL, Pm4 to powdery mildew on 2AL, Yr2, Yr9, Sr 31 and Lr26 and a new Yr to stripe rust on 7B, 1BL, 1RS and 2BL. Restriction fragment length polymorphism (RFLP) markers Xpsr687 and Xwg380 , sequence tagged site (STS) marker STS 1700 , simple sequence repeat (SSR) markers Xgwmc364 and Xgwm582 , SSR markers Xgwm388 and Xgwm501 can be used as diagnostic tools to track Bdv2, Pm4, Yr2, Yr9 and Yr in YW243 , respectively; and two amplified fragment length polymorphism (AFLP) markers M54E63 - 700 and M54E64 - 699 can also be used to select Yr in YW243 .

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Summary

The chemical compositions of essential oils extracted by n-hexane extract (HE), petroleum ether extract (PE), dichloromethane extract (DE), and hydrodistillation (HD) from Carthamus tinctorius L. (safflower) were analyzed by gas chromatography-mass spectrometry (GC-MS). A total of 86 compounds from four different extracts were identified, and the contents were 97.65%, 98.05%, 98.93%, and 99.68%, respectively. 6,10,14-Trimethyl-2-pentadecanone, hexadecanoic acid, methyl ester, hexadecanoic acid, 8,11-octadecadienoic acid, methyl ester, and 9,12,15-octadecatrien-1-ol were the major constituents of the extracts. The antidiabete activity was assayed in vitro by against protein tyrosine phosphatase 1B (PTP1B). The results showed that the HE exhibited the best in vitro inhibitory enzyme activity against PTP1B, which holds a good potential for treating diabetes and obesity.

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Abstract  

The migration of 99Tc in a weak loess aquifer was investigated in-situ with undisturbed aquifer medium columns. The columns were obtained horizontally at a depth of 3236 m in an Underground Research Facility (URF). Quartz containing 3H (HTO) and 99Tc (in the form of 99TcO4 -) was introduced into one end of the columns and the columns were covered tightly. Aquifer water was introduced into the columns directly from an experimental shaft in the UFR. Effluents from the columns were collected and the activity of 3H and 99Tc were determined with a liquid scintillation analyzer. The breakthrough curves of 3H and 99Tc indicate that 99Tc migrates a little faster than that 3H does in the aquifer.

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Abstract  

The migration of 99Tc in unsaturated Chinese loess was investigated in-situ with a tracer method. Quartz containing 3H (HTO) and 99Tc (99TcO4 -) was introduced into the bottom of an experimental pit which was then backfilled at the field test site. Then core soil samples were taken and cut vertically into 1 cm long slices. The slice samples were analyzed by liquid scintillation techniques in the laboratory. The results indicate that the migration pattern of 99Tc was quite similar to that of 3H and the vertical diffusion coefficients of 99Tc and 3H were calculated as (4.7±0.4).10-2 cm2/d and (7.8±0.4).10-2 cm2/d, respectively.

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Cereal Research Communications
Authors:
W.F. Song
,
Z.Y. Ren
,
Y.B. Zhang
,
H.B. Zhao
,
X.B. Lv
,
J.L. Li
,
C.H. Guo
,
Q.J. Song
,
C.L. Zhang
,
W.L. Xin
, and
Z.M. Xiao

Two lines, L-19-613 and L-19-626, were produced from the common wheat cultivar Longmai 19 (L-19) by six consecutive backcrosses using biochemical marker-assisted selection. L-19 (Glu-D1a, Glu-A3c/Gli-A1?; Gli-A1? is a gene coding for unnamed gliadin) and L-19-613 (Glu-D1d, Glu-A3c/Gli-A1?) formed a set of near-isogenic lines (NILs) for HMW-GS, while L-19-613 and L-19-626 (Glu-D1d, Glu-A3e/Gli-A1m) constituted another set of NILs for the LMW-GS/gliadins. The three L-19 NILs were grown in the wheat breeding nursery in 2007 and 2008. The field experiments were designed using the three-column contrast arrangement method with four replicates. The three lines were ranked as follows for measurements of gluten strength, which was determined by the gluten index, Zeleny sedimentation, the stability and breakdown time of the farinogram, the maximum resistance and area of the extensogram, and the P andWvalues of the alveogram: L-19-613 > L-19-626 > L-19. The parameters listed above were significantly different between lines at the 0.05 or 0.01 level. The Glu-D1 and Glu-A3/Gli-A1 loci had additive effects on the gluten index, Zeleny sedimentation, stability, breakdown time, maximum resistance, area, P and W values. Although genetic variation at the Glu-A3/Gli-A1 locus had a great influence on wheat quality, the genetic difference between Glu-D1d and Glu-D1a at the Glu-D1 locus was much larger than that of Glu-A3c/Gli-A1? and Glu-A3e/Gli-A1m at the Glu-A3/Gli-A1 locus. Glu-D1d had negative effects on the extensibility and the L value compared with Glu-D1a. In contrast, Glu-A3c/Gli-A1? had a positive effect on these traits compared with Glu-A3e/Gli-A1m.

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