Dynamic mechanical relaxation and thermal creep of high-entropy La30Ce30Ni10Al20Co10 bulk metallic glass

Spatial frequency shift(SFS) microscopy with evanescent wave illumination shows intriguing advantages, including large field of view(FOV), high speed, and good modularity. However, a missing band in the spatial frequency domain hampers the SFS superresolution microscopy from achieving resolution better than 3 folds of the Abbe diffraction limit. Here, we propose a novel tunable large-SFS microscopy, making the resolution improvement of a linear system no longer restricted by the detection numerical aperture(NA). The complete wide-range detection in the spatial frequency domain is realized by tuning the illumination spatial frequency actively and broadly through an angle modulation between the azimuthal propagating directions of two evanescent waves. The vertical spatial frequency is tuned via a sectional saturation effect, and the reconstructed depth information can be added to the lateral superresolution mask for 3D imaging. A lateral resolution of λ/9, and a vertical localization precision of ~λ/200(detection objective NA = 0.9) are realized with a gallium phosphide(GaP) waveguide. Its unlimited resolution enhancing capability is demonstrated by introducing a designed metamaterial chip with an unusual large refractive index. Besides the great resolution enhancement, this method shows better anti-noise capability than classical structured illumination microscopy without SFS tunability. This method is chip-compatible and can potentially provide a massproducible illumination chip module achieving the fast, large-FOV, and deep-subwavelength 3D nanoscopy.     

基质辅助激光解析电离质谱和电喷雾质谱共同快速确证达托霉素结构

运用基质辅助激光解析电离-飞行时间串联质谱(MALDI-TOF/TOF MS)和电喷雾-四级杆-飞行时间质谱(ESI-Q-TOF MS)快速确证环脂肽达托霉素的结构。首先,ESI检测达托霉素相对分子量为1619.7107,与理论值偏差0.0007。选择其双电荷峰m/z 809.848作为母离子进行ESI串联质谱(MS/MS)测定,成功匹配了达托霉素环外氨基酸序列C9H19CO-Trp-Asn-Asp。其次,优化Li OH裂解达托霉素的实验条件,以MALDITOF/TOF MS监测开环效果,获得95%以上的开环样本后,分别运用MALDI和ESI进行MS/MS测定,达托霉素开环产物的b+和y+全部被匹配,达托霉素全部氨基酸序列得到确证。最后,对开环产物的ESI-MS/MS条件进一步优化,获得了丰富的低端碎片离子,解析了脂肪酸链结构,并绘制了脂肪酸链的裂解图。本方法快速、简便、准确,是确证环脂肽类化合物结构的可靠方法。     

Ultra-sensitive quantification of lysozyme based on element chelate labeling and capillary electrophoresis–inductively coupled plasma mass spectrometry

In this study, an ultra-sensitive method for the quantification of lysozyme based on the Gd³⁺ diethylenetriamine-N,N,N′,N″,N″-pentaacetic acid labeling and capillary electrophoresis–inductively coupled plasma mass spectrometry (CE–ICP–MS) was described. The Gd³⁺-tagged lysozyme was effectively separated by capillary electrophoresis (CE) and sensitively determined by inductively coupled plasma mass spectrometry (ICP–MS). Based on the gadolinium-tagging and CE–ICP–MS, the lysozyme was determined within 12 min with an extremely low detection limit of 3.89 attomole (3.89 × 10⁻¹¹ mol L⁻¹ for 100 nL of sample injection) and a RSD < 6% (n = 5). The proposed method has been successfully used to detect lysozyme in saliva samples with a recovery of 91–106%, suggesting that our method is sensitive and reliable. The success of the present method provides a new potential for the biological assays and sensitive detection of low-abundant proteins.     

The emission positions of kHz QPOs and Kerr spacetime influence

Based the Alfven wave oscillation model (AWOM) and relativistic precession model (RPM) for twin kHz QPOs, we estimate the emission positions of most detected kHz QPOs to be at r=18+/−3 km (R/15 km), except Cir X-1 at r∼30+/−5 km (R/15 km). For the proposed Keplerian frequency as an upper limit to kHz QPO, the spin effects in Kerr Spacetime are discussed, which have about a 5% (2%) modification for that of the Schwarzchild case for the spin frequency of 1000 (400) Hz. The application to the four typical QPO sources, Cir X-1, Sco X-1, SAX J1808.4-3658 and XTE 1807-294, is mentioned.

     

The time lag spectrum of Cir X-1 on its normal branch

In the radiation-hydrodynamics model, the time lag and fractional root-mean-squared (rms) amplitude as a function of emitted photon energy should show a minimum on the normal branch oscillations. This has been seen in the Z-sources Cyg X-2 and GX 5-1. Here, using the observations from the Rossi X-ray Timing Explorer (RXTE), we study the energy dependence of normal branch QPOs in the peculiar Z-source Cir X-1. We discuss the results in the context of radiation-hydrodynamics and the Comptonization model.     

三线性分解方法用于激发-发射矩阵荧光数据中一阶瑞利散射的扣除

由于荧光分析具有检测灵敏度高、数据容易获得等优点,近年来二阶张量校正方法与激发-发射矩阵荧光光谱技术的联用正受到人们越来越多的关注.但是,在三维荧光分析中,经常出现的一阶瑞利散射干扰往往容易导致建立的三线性模型存在较大的偏离,进而直接影响复杂体系中感兴趣组分的定性、定量分析.针对该问题,我们提出了一种基于对组分数不敏感的三线性分解算法扣除一阶瑞利散射干扰的新思路.该方法的特点是根据一阶瑞利散射分别在水平切片矩阵和侧面切片矩阵所处位置相同,沿I-模和J-模同时构建含一阶瑞利散射的三维数据阵,利用三线性分解算法对此各自建模,将一阶瑞利散射当作一个响应组分或因子拟合后从三维数据阵中扣除掉.通过对模拟和实际三维激发发射矩阵荧光光谱实验数据进行讨论,结果表明该方法能有效地扣除体系中的一阶瑞利散射干扰.改进后的方法不仅操作简单,而且不受组分数选取不当的困扰.另外,由于同时从两个方向进行一阶瑞利散射扣除,因此不会出现因边缘瑞利散射峰形不完整而扣除不完全的情况.该方法为三维荧光光谱的无损分析提供了新思路,为进一步进行三维荧光光谱的定量分析奠定了良好的基础.     

The rms-flux relation of Cyg X-2 in the horizontal branch

We have investigated the relation between the root mean square (rms) variability and the X-ray flux (rms-flux relation) of the Z source Cyg X-2, and as well the energy dependence based on the Rossi X-ray Timing Explorer (RXTE) observations. We currently focus on the horizontal branch (HB), due to the negative correlation in flux of the soft and the hard X-rays. The rms-flux correlation has energy dependence as follows: positive at hard X-rays (above 10 keV) but negative at soft X-rays (below 10 keV). This provides a feature different from the previous one, and may be suggestive of different origins of X-rays below and above 10 keV. Nevertheless, the overall spectrum can be well fitted with a model consisting of a blackbody and Comptonization components, but the fitting results do not reveal any features around 10 keV that could account for such a change in the rms-flux relation.     

A “turn-on” and label-free fluorescent assay for the rapid detection of exonuclease III activity based on Tb3+-induced G-quadruplex conjugates

A “turn-on” and label-free fluorescent assay for the specific, rapid, and sensitive detection of 3′?→?5′ exonuclease III activity is reported in this study. The assay is based on the Tb³⁺-promoted G-quadruplex, which lead to the enhancement of Tb³⁺ fluorescence due to the energy transfer from guanines. The proposed assay is highly simple, rapid, and cost-effective, and does not require sophisticated experimental techniques such as gel-based equipment or radioactive labels. It can be used for the rapid detection of exonuclease III activity with a detection limit of 0.8 U and a RSD (n?=?6) <5 %. Notably, no dye was covalently conjugated to the DNA strands, which offers the advantages of low-cost and being interference-free.