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BODIPY-based chemosensors are widely used owing to merits like good selectivity, high fluorescence quantum yield, and excellent optical stability. As such, a pH-switchable hydrophilic fluorescent probe, BODIPY-PY-(SO3Na)2, was developed for detection of Fe3+ ion in aqueous solutions. BODIPY-PY-(SO3Na)2 revealed strong fluorescence intensity and was responsive to pH value in the range of 6.59-1.96. Additionally, BODIPY-PY-(SO3Na)2 showed good selectivity and sensitivity towards Fe3+. A good linear relationship for Fe3+ detection was obtained from 0.0 µM to 50.0 µM with low detecting limit of 6.34 nM at pH 6.59 and 2.36 nM at pH 4.32, respectively. The response to pH and detection of Fe3+ induced obvious multicolor changes. BODIPY-PY-(SO3Na)2 can also be utilized to quantitatively detect Fe3+ in real water sample. Different mechanisms of Fe3+ detection at investigated pH values were unraveled through relativistic density functional theory (DFT) calculations in BODIPY-PY-(SO3Na)2 and experiments of coexisting cations, anions and molecules. These results enabled us to gain a deeper understanding of the interactions between BODIPY-PY-(SO3Na)2 and Fe3+ and provide valuable fundamental information for design of efficient multicolor chemosensors for Fe3+ as well.
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Optical switches are increasingly acknowledged for their potential advantages over mechanical counterparts in various domains. However, research on optical switches remains relatively nascent, primarily focusing on applications like anti-counterfeiting, switching chemical reactions, etc., while neglecting the control of photocurrent switching. Here, we have developed NaYF4:30 %Er-NaYF4-NaYF4:20 %Ho-NaYF4 core-shell nanocrystals with unique upconversion (UC) multi-color emission properties under 1530 nm, 980 nm and 1150 nm laser excitations. These nanocrystals allow for optical control of circuit switching by modulating photocurrent signals in photosensitive circuits. The UC emission is due to the self-sensitization of rare earth ions in the core and shell. By adjusting the intermediate shell thickness, we have optimized the luminescence and investigated the mechanism. Combining these nanocrystals with a WO3 quantum dots (QDs) photochromic hydrogel, dynamic variation of UC emissions could be realized. Moreover, by combining with a commercial silicon photodetector, we constructed a photosensitive circuit demonstrating the modulation of photocurrent signal output and realized the "hard switching" of rapid circuit cutoff. Furthermore, by using the photochromic effect of WO3 QDs, the "soft switching" of slow circuit cutoff and recovery were also achieved. This work has significant implications for the development and application such as energy management system and smart home of optical switches in various fields.
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Multi-mode dynamic anti-counterfeiting materials can provide complex anti-counterfeiting performance and ensure the anti-counterfeiting strategy becomes more secure. Herein, a new type of multi-mode anti-counterfeiting encryption material of CaAl12O19:Eu, Er with different Er doping concentration was developed by sol-gel method. Interestingly, the CaAl12O19:Eu, Er phosphor and its composite have multi-mode anti-counterfeiting characteristics of multi-color down-conversion luminescence, up-conversion luminescence, dynamic luminescence, and photochromism. Effect of different Er doping concentration on the down-conversion luminescence, up-conversion luminescence, dynamic luminescence, and photochromism of CaAl12O19:Eu, Er was systematically investigated, and the relevant mechanisms were discussed. These anti-counterfeiting features can be simultaneously applied in both bright and dark fields, which can achieve high-level anti-counterfeiting in both spatial and temporal dimensions. The CaAl12O19:Eu, Er phosphors cannot be easily replaced by other materials with the same anti-counterfeiting properties. They display good application foreground in the field of anti-counterfeiting encryption.
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Conjugated polymer electrochromic materials (PECMs) with tailored optical and electrical properties are applied in smart windows, electronic displays, and adaptive camouflage. The limitation in the electrical conductivity results in slow and monotonous color switching. We present a polypyrrole film incorporated with a toluene-p-sulfonic group (PPy-TSO-F), via a one-step electrodeposition technique. The PPy-TSO-F thin film (110 nm) achieves an impressive electrical conductivity of 1011 S cm-1, a high carrier mobility of 82 cm2 V-1 s-1, and intrinsic metallic electronic behavior. It demonstrates exceptionally reversible multicolor switching, transitioning from emerald green (-1.5 V), to bluish green (-1.4 V), bright yellow (-1.2 V), greenish yellow (-0.6 V), reddish brown (0.1 V), dark brown (0.3 V), and atrovirens (0.6 V). The fast charge transport and high carrier mobility render the film with an ultrafast electrochromic switching speed of 0.01 s/0.02 s. This research provides a new route to designing ultrafast multicolor switching PECMs with metallic charge transport.
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Aggregation-induced emission (AIE) carbon dot (CDs) in solid state with tunable multicolor emissions have sparked significant interest in multidimensional anti-counterfeiting. However, the realization of solid-state fluorescence (SSF) by AIE effect and the regulation of fluorescence wavelength in solid state is a great challenge. In order to solve this dilemma, the AIE method to prepare multi-color solid-state CDs with fluorescence wavelengths ranging from bright blue to red emission is employed. Specifically, by using thiosalicylic acid and carbonyl hydrazine as precursors, the fluorescence wavelength can be accurately adjusted by varying the reaction temperature from 150 to 230 °C or changing the molar ratio of the precursors from 1:1 to 1:2. Structural analysis and theoretical calculations consistently indicate that increasing the sp2 domains or doping with graphite nitrogen both cause a redshift in the fluorescence wavelength of CDs in the solid state. Moreover, with the multi-dimensional and adjustable fluorescence wavelength, the application of AIE CDs in the fields of multi-anti-counterfeiting encryption, ink printing, and screen printing is demonstrated. All in all, this work opens up a new way for preparing solid-state multi-color CDs using AIE effect, and further proposes an innovative strategy for controlling fluorescence wavelengths.
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Utilizing a single organic light-emitting diode (OLED) architecture for multicolor emissions can significantly simplify manufacturing progress and broaden applications. Here, we report on a carbene-based Pt(II) complex, designated as Pt(pyiOppy), which exhibits an unusual dimeric packing mode solely by hemiligand π···π stacking. This feature is distinct from the well-known Pt···Pt or Pt···ligand interactions. The dimer persists in new types of orbital combinations, along with its triplet transition state, which are evidenced for the first time. Pt(pyiOppy), under various doping concentrations in a solid matrix, demonstrates multicolor emissions ranging from green to red, all exhibiting high photoluminescent quantum efficiencies (48-97%). The devices incorporating Pt(pyiOppy) can emit green, yellow, orange, and red lights, covering a CIE coordinate range of (0.28-0.65, 0.61-0.34). All the devices also achieve appreciable maximum external quantum efficiencies (9.4-17.2%) and impressive lifetimes of hundreds of hours (LT70 at 1000 cd/m2). These findings showcase a new type of Pt(II) aggregate enabling well-controlled, multicolor high-performance phosphorescent OLEDs.
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Excessive reactive oxygen species (ROS) in seminal plasma can trigger male infertility. Therefore, the development of simple and rapid ROS detection methods is urgently needed, particularly for the early self-screening of preconception couples. Herein, a gold nanobipyramid (Au NBP)-based colorimetric hydrogel for convenient and fast ROS detection is described. In the hydrogel, Au NBP is etched efficiently by ROS under the synergistic effect of Fe2+and I-, which finally causes color variations. Besides, agarose gel with the function of molecular sieve enables the separation of biomacromolecules, improving the interference resistance of the system and the stability of Au NBP. This chemical sensor can complete all the tests within 20 min, covering two detection range of 10-125 µM at relative low H2O2 concentration and 125-1000 µM at relative high H2O2 concentration, with the detection limits of 1.76 µM and 12.10 µM (S/N = 3) respectively. Furthermore, via visual observation of the color variations, it allows the initial interpretation of ROS concentration without any additional equipment. We applied this device to the detection of ROS in clinical seminal plasma samples and obtained promising results, demonstrating its potential for rapid and convenient detection in clinical applications.
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A capsaicinoids (CPCs) broad spectrum monoclonal antibody with same recognition ability to capsaicin (CPC), dihydrocapsaicin (DCPC), nordihydrocapsaicin (NDCPC), and N-vanillylnonanamide (NV) is prepared. Chitosan (CS) hydrogel is used as the carrier of multicolor quantum dots (QDs) to prepare fluorescence hydrogel beads, CPCs and aflatoxin B1 (AFB1) antibody are coupled with fluorescence hydrogel beads to prepare signal probes. Using AuNPs (or AgNPs) as fluorescence quenching agent to prepare quenching probes followed forming a fluorescence quenching test system. Based on optimal group of signal and quenching probes, a novel, simple, convenient, and ultra-sensitive homogeneous fluorescence immunoassay for the simultaneous detection of CPCs and AFB1 is constructed. The limit of detection (LOD) of assay for AFB1 and CPC is 0.00064 µg L-1 and 0.00049 µg L-1, respectively. This method can realize the simultaneous rapid detection of AFB1 and CPCs in food, which provides a new strategy for the identification of kitchen waste oil.
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Carbon dots (CDs) offer tremendous advantages in the fields such as bioimaging, sensing, biomedicine, catalysis, information encryption, and optoelectronics. However, the inherent challenge is synthesizing CDs with a full-spectrum emission, as most CDs typically produce only blue or green emissions, which severely hinder further investigation into their fluorescence mechanism and restrict their broader applications in light-emitting diodes (LEDs). In this work, we reported a solvent-controlled strategy for the preparation of multicolor CDs with blue, yellow, and red emissions, using o-phenylenediamine (oPD) and ionic liquid 1-butyl-3-methylimidazolium hexafluorophosphate (BmimPF6) as precursors. The detailed characterizations proved that a solvent with a lower boiling point and lower solubility of precursors resulted in a higher degree of dehydration and carbonization process, thereby increasing carbon cores with sp2-conjugated domains and nitrogen doping and further reducing the bandgap energies, causing a significant redshift emission from blue to red. The underlying fluorescence mechanism of the prepared multicolor CDs was contributed to the surface state. Eventually, blue-, yellow-, and red-emitting CDs based on poly(vinyl alcohol) (PVA) films and colorful LEDs devices were fabricated by dispersing the as-synthesized CDs into a PVA solution. The proposed solvent-controlled strategy for multicolor CDs preparation will be helpful for fully utilizing the advantages of CDs and expanding their applications.
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Candida albicans is the most common human fungal pathogen, able to reside in a broad range of niches within the human body. Even though C. albicans systemic infection is associated with high mortality, the fungus has historically received relatively little attention, resulting in a lack of optimized molecular and fluorescent tools. Over the last decade, some extra focus has been put on the optimization of fluorescent proteins (FPs) of C. albicans. However, as the FPs are GFP-type, they require an aerobic environment and a relatively long period to fully mature. Recently, we have shown the application of a novel type of fluorogen-based FP, with an improved version of fluorescence activating and absorption shifting tag (iFAST), in C. albicans. Due to the dynamic relation between iFAST and its fluorogens, the system has the advantage of being reversible in terms of fluorescence. Furthermore, the combination of iFAST with different fluorogens results in different spectral and cellular properties, allowing customization of the system. Key features ⢠Genetic integration and tagging with the iFAST tag in Candida albicans. ⢠Imaging and localization of a protein of interest tagged with iFAST. ⢠Reversibility of fluorescence with iFAST.
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In the context of high-grade gliomas such as glioblastoma (GBM), the immune part of the tumor microenvironment (TME) is involved in tumor growth and tumor recurrence. It is mostly represented by high amount of macrophages and low amount of lymphocytes. GBM in itself as well as x-ray-based radiotherapy, a standard treatment for brain tumors, are also associated with systemic effects like lymphopenia that correlates with a poor prognosis. This contributes to the immune-suppressive nature of the TME and may explain the lack of the anti-tumor immune response. Radiation-induced lymphopenia (RIL) is generally evaluated on CD4+ and CD8+ count or on a CBC (complete blood count), but the heterogeneity of the subtypes prompts us to explore them in detail to better understand the cellular response to brain irradiation. To facilitate and develop the evaluation of x-ray brain exposure on circulating immune cells, we developed a reproducible and reliable method to quantify the variation of lymphoid and myeloid subtypes using flow cytometry after brain irradiation in the rodent.
Asunto(s)
Neoplasias Encefálicas , Encéfalo , Citometría de Flujo , Animales , Citometría de Flujo/métodos , Ratones , Encéfalo/patología , Encéfalo/efectos de la radiación , Neoplasias Encefálicas/radioterapia , Neoplasias Encefálicas/patología , Leucocitos/efectos de la radiación , Microambiente Tumoral/inmunología , Glioblastoma/radioterapia , Glioblastoma/patología , Glioblastoma/inmunología , Glioblastoma/sangre , Linfopenia/etiología , Linfopenia/patología , Linfopenia/sangreRESUMEN
In vulnerable atherosclerotic plaques, intraplaque hemorrhages (IPH) result in hemolysis of red blood cells and release of hemoglobin and free hemin. Hemin activates platelets and leads to thrombosis. Agonism of the inhibitory platelet receptor ACKR3 inhibits hemin-dependent platelet activation and thrombus formation. To characterize the effect of hemin and ACKR3 agonism on isolated human platelets, multi-color flow cytometry and classical experimental setup such as light transmission aggregometry and a flow chamber assay were used. Hemin induces platelet aggregation and ex vivo platelet-dependent thrombus formation on immobilized collagen under a low shear rate of 500 s-1, indicating that free hemin is a strong activator of platelet-dependent thrombosis. Recently, we described that ACKR3 is a prominent inhibitory receptor of platelet activation. Specific ACKR3 agonists but not conventional antiplatelet compounds such as COX-1 inhibitor (indometacin), ADP-receptor blocker (cangrelor), or PAR1 inhibitor (ML161) inhibit both hemin-dependent aggregation and thrombus formation. To further characterize the effect of hemin on platelet subpopulations, we established a multi-color flow cytometry assay. We found that hemin induces procoagulant (CD42bpos/PAC-1neg/AnnexinVpos), aggregatory (CD42bpos/PAC-1pos/AnnexinVneg), and inflammatory (CD42bpos/CXCR4pos/ACKR3pos/AnnexinVpos) platelet subpopulations. Treatment with ACKR3 agonists significantly decreased the formation of procoagulant and ACKR3pos platelets in response to hemin. We conclude that hemin is a strong activator for the formation of procoagulant platelets and thrombus formation which is dependent on the function of ACKR3. Activation of ACKR3 using specific agonists may offer a therapeutic strategy to regulate the vulnerability of atherosclerotic plaques in areas of IPH.
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In this work, oleic acid (OA)-capped core-heptad-shell (CHS) nanocrystals (NCs) that exhibit multiple emissions achieved through downshifting and orthogonal upconversion are synthesized via layer-by-layer thermal decomposition. This method enables the downshifting process to be accommodated by doping ions in the inert space between two upconversion patterns (the core and fourth shell) and doping Ce/Tb or Ce/Eu ions in the NaGdF4 layer for the first time. These developed CHS NCs exhibit different emission colors via 980 and 800 nm orthogonal upconversion and downshifting emissions under 256 nm UV excitation in hexane solvent. Furthermore, surface-functionalized OA is removed using mild acid treatment. The resulting bare CHS NCs disperse well in water and exhibit 21.60-fold and 43.59-fold higher Ce/Tb and Ce/Eu luminescence intensities, respectively, than the OA-capped CHS NCs. These NCs are mixed with a carboxymethylcellulose (CMC) polymer in an aqueous medium to form a CMC-CHS NC gel. Invisible patterns and QR codes are printed on nonfluorescent paper using gels and screen-printing techniques. These patterns and QR codes exhibit three different emission colors under three different excitations. This method can be used for high-level anticounterfeiting applications.
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Host-guest chemistry of chiral metal-organic frameworks (MOFs) has endowed them with circularly polarized luminescence (CPL), it is still limited for MOFs to systematically tune full-color CPL emissions and sizes. This work directionally assembles the chiral ligands, metal sites and organic dyes to prepare a series of crystalline enantiomeric D/L-Cd/Zn-n MOFs (n=1~5, representing the adding amount of dyes), where D/L-Cd/Zn with the formula of Cd2(D/L-Cam)2(TPyPE) and Zn2(D/L-Cam)2(TPyPE) (D/L-Cam=D/L-camphoric acid, TPyPE=4,4',4'',4'''-(1,2-henediidenetetra-4,1-phenylene)tetrakis[pyridine]) were used as the chiral platforms. The framework-dye-enabled emission and through-space chirality transfer facilitate D/L-Cd/Zn-n bright full-color CPL activity. The ideal yellow CPL of D-Cd-5 and D-Zn-4, with |glum| as 4.9 × 10-3 and 1.3×10-3 and relatively high photoluminescence quantum yield of 40.79 % and 45.40 %, are further assembled into a white CPL light-emitting diode. The crystal sizes of D/L-Cd/Zn-n were found to be strongly correlated to the types and additional amounts of organic dyes, that the positive organic dyes allow for the preparation of > 7â mm bulks and negative dyes account for sub-20â µm particles. This work opens a new avenue to fabricate full-color emissive CPL composites and provides a potentially universal method for controlling the size of optical platforms.
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In this study, we demonstrated an approach for the development of multiplex immunochromatographic test strip (MICS) for neomycin (NEO), penicillin (PEN), and chloramphenicol (CAP) detection using three different-colored gold nanoparticles. The gold nanoparticles: gold nanospheres (red), gold nanostars (blue), and gold nanoflowers (black) were applied as labels for MICS fabrication. The proposed MICS achieved a clearly visible limit of detection with cut-off values of 500, 5, and 0.5 µg L-1 for NEO, PEN, and CAP, respectively within only 10 min. Such smartphone-based detection provided a limit of detection of 3.70 µg L-1 for NEO, 0.10 µg L-1 for PEN, and 0.008 µg L-1 for CAP. The analysis of real samples by the developed MICS was well correlated with the enzyme-linked immunosorbent assay and liquid chromatography-mass spectrometry. The proposed MICS has the potential to be used for the simultaneous detection of NEO, PEN, and CAP with rapid, precise, and sensitive results.
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The ultimate miniaturization of any optical system relies on the reduction or removal of free-space gaps between optical elements. Recently, nonlocal flat optic components named "spaceplates" were introduced to effectively compress space for light propagation. However, space compression over the visible spectrum remains beyond the reach of current spaceplate designs due to their inherently limited operating bandwidth and functional inefficiencies in the visible range. Here, we introduce "multi-color" spaceplates performing achromatic space compression at three distinct color channels across the visible spectrum to markedly miniaturize color imaging systems. In this approach, we first design monochromatic spaceplates with high compression factors and high transmission amplitudes at visible wavelengths based on a scalable structure and dielectric materials widely used in the fabrication of meta-optical components. We then show that the dispersion-engineered combination of monochromatic spaceplates with suitably designed transmission responses forms multicolor spaceplates that function achromatically. The proposed multicolor spaceplates, composed of amorphous titanium dioxide and silicon dioxide layers, efficiently replace free-space volumes with compression ratios as high as 4.6, beyond what would be achievable by a continuously broadband spaceplate made of the same materials. Our strategy for designing monochromatic and multicolor spaceplates, along with the presented theoretical and computational results, show that strong space-compression effects can be achieved in the visible range. Our findings may ultimately enable a new generation of ultrathin optical devices for various applications.
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Paper-based cultural relics often undergo acidification and deterioration during long-term preservation. Accurate detection of paper acidity is of great significance to assess aging status and extend the preservation lifetime of paper-based cultural relics. Rapid identification of the acidification degree and acid distribution across multiple regions of paper is essential. Inspired by fluorescent sensing technology, pH-sensitive cadmium telluride (CdTe) quantum dots (QDs) and rhodamine B (RB) fluorescent probes are synthesized and incorporated onto the nanofibers of a bacterial cellulose (BC) membrane to enable visual acidity detection of paper. Due to the complementary pH detection range of CdTe QDs and RB probes, the composite BC membrane exhibits a clear pH response across an acidic to neutral range (pH 3.0-7.5). Notably, the contrasting fluorescent colors of the two probes within the BC membrane allow for easy visualization of paper pH and acidity distribution with the naked eyes. A distinct color transition from red to green was observed on the fluorescent BC membrane when it is applied to a model paper with a gradient pH distribution. The feasibility of this method was verified by using the flat-headed pH electrode method. Additionally, common metal ions in most paper fillers, inks, pigments, as well as some sugars and amino acids showed minimal interference with the pH response of the composite BC membrane, highlighting its potential and broad applicability for visual acidity detection in paper-based cultural relics.
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Understanding the localization and the interactions of biomolecules at the nanoscale and in the cellular context remains challenging. Electron microscopy (EM), unlike light-based microscopy, gives access to the cellular ultrastructure yet results in grey-scale images and averts unambiguous (co-)localization of biomolecules. Multimodal nanoparticle-based protein labels for correlative cathodoluminescence electron microscopy (CCLEM) and energy-dispersive X-ray spectromicroscopy (EDX-SM) are presented. The single-particle STEM-cathodoluminescence (CL) and characteristic X-ray emissivity of sub-20 nm lanthanide-doped nanoparticles are exploited as unique spectral fingerprints for precise label localization and identification. To maximize the nanoparticle brightness, lanthanides are incorporated in a low-phonon host lattice and separated from the environment using a passivating shell. The core/shell nanoparticles are then functionalized with either folic (terbium-doped) or caffeic acid (europium-doped). Their potential for (protein-)labeling is successfully demonstrated using HeLa cells expressing different surface receptors that bind to folic or caffeic acid, respectively. Both particle populations show single-particle CL emission along with a distinctive energy-dispersive X-ray signal, with the latter enabling color-based localization of receptors within swift imaging times well below 2 min per µ m $\umu\text{m}$ 2 while offering high resolution with a pixel size of 2.78 nm. Taken together, these results open a route to multi-color labeling based on electron spectromicroscopy.
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High-grade B-cell lymphomas (HGBCL) represent a heterogeneous group of very rare mature B-cell lymphomas. The 4th revised edition of the WHO Classification of Tumors of Hematopoietic and Lymphoid Tissues (WHO-HAEM) previously defined two categories of HGBCL: the so-called double-hit (DHL) and triple-hit (THL) lymphomas, which were related to forms harboring MYC and BCL2 and/or BCL6 rearrangements, and HGBCL, NOS (not otherwise specified), corresponding to entities with intermediate characteristics between diffuse large B-cell lymphoma (DLBCL) and Burkitt lymphoma (BL), without rearrangement of the MYC and BCL2, and/or BCL6 genes. In the 5th edition of the WHO-HAEM, DHL with MYC and BCL2 rearrangements or THL were reassigned as DLBCL/HGBCL with MYC and BCL2 rearrangements (DLBCL/HGBL-MYC/BCL2), whereas the category HGBCL, NOS remains unchanged. Characterized by an aggressive clinical presentation and a poor prognosis, HGBCL is often diagnosed at an advanced, widespread stage, leading to potential disseminated forms with a leukemic presentation, or spreading to the bone marrow (BM) or other biological fluids. Flow cytometric immunophenotypic study of these disseminated cells can provide a rapid method to identify HGBCL. However, due to the scarcity of cases, only limited data about the immunophenotypic features of HGBCL by multiparametric flow cytometry are available. In addition, identification of HGBCL cells by this technique may be challenging due to clinical, pathological, and biological features that can overlap with other distinct lymphoid malignancies, including Burkitt lymphoma (BL), diffuse large B-cell lymphoma (DLBCL), and even B acute lymphoblastic leukemia (B-ALL). In this study, we aimed to characterize the detailed immunophenotypic portrait of HGBCL, evaluating by multiparametric flow cytometry (MFC) the expression of 26 markers on biological samples obtained from a cohort of 10 newly-diagnosed cases and comparing their level of expression with normal peripheral blood (PB) B lymphocytes (n = 10 samples), tumoral cells from patients diagnosed with B-ALL (n = 30), BL (n = 13), or DLBCL (n = 22). We then proposed a new and simple approach to rapidly distinguish disseminated forms of HGBCL, BL, and DLBCL, using the combination of MFC data for CD38, BCL2, and CD39, the three most discriminative markers explored in this study. We finally confirmed the utility of the scoring system previously proposed by Khanlari to distinguish HGBCL cells from B lymphoblasts of B-ALL. In conclusion, we described a distinct immunophenotypic portrait of HGBCL cells and proposed a strategy to differentiate these cells from other aggressive B lymphoma entities in biological samples.
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The development of an affordable, portable, and instrument-free colorimetric biosensor holds significant importance for routine monitoring and clinical diagnosis. To overcome the limitations that traditional monochromatic colorimetric kits struggle to distinguish subtle color changes with the naked eye, we designed and constructed a portable hydrogel kit for polychromatic semi-quantitative and quantitative sensing analysis. When the actual samples and I- were introduced into a gelatin hydrogel encapsulated with MIL-88A(Fe), Au NRs and oxidase (Au@GM88A/I), a noticeable color change occurred. Additionally, a mathematic model between Hue and multicolor signal was set up for the first time by mobile phone photo technology, successfully applied to the glucose detection in serum. The visual detection had a wide concentration range of 0.02-0.80â¯mM with a limit of detection down to 0.02â¯mM. Above all, hydrogel kit prepared with gelatin as a carrier addressed the issues of uneven color and slow response rate commonly seen in gels like sodium alginate and agarose. This improvement would be beneficial for enhancing the accuracy of color captured by mobile phone assisted hydrogel kits, making it a valuable tool for biomarker analysis.