الملخص
Objective To investigate the effect of4-amino-2-trifluoromethyl-phenyl retinate(ATPR)on acute liver injury induced by lipopolysaccharide(LPS)in C57BL/6 mice and its related mechanism.Methods Fifteen 6-week-old male C57BL/6 strain mice were randomly divided into normal group,model group and ATPR group,with 5 mice in each group.Mice in the ATPR group were intraperitoneally injected with ATPR(15 mg/kg·d),and normal group and model group were given solvent.After continuous administration for one week,model group and ATPR group were intraperitoneally injected with LPS(6 mg/kg),and all mice were sacrificed 6 hours later.The contents of Alanine aminotransferase(ALT)and Aspartate aminotransferase(AST)in serum of mice were detec-ted.The mRNA levels of Interleukin-6(IL-6)and Tumor necrosis factor-alpha(TNF-α)were detected by qPCR.Hematoxylin-eosin(H&E)staining was used to observe the histopathological changes of liver in mice.The ultra-structural changes of mouse hepatocytes were observed by Transmission electron microscope(TEM).The expres-sion levels of mitochondrial damage-related proteins FUNDC1 and OPA1 and autophagy related proteins LC3B,P62,Beclin1 and ATG5 were detected by Western blot.Results Compared with the normal group,the content of ALT and AST in serum and the mRNA levels of IL-6 and TNF-α in liver tissue increased in the model group,and the changes were reversed in the ATPR group.H&E staining showed that the hepatic lobule structure was normal in the normal group,the hepatic cords were arranged radially,there was no hyperemia and inflammatory cell infiltra-tion,and the hepatocyte boundary was clear.In the model group,the intercellular space of liver was enlarged,the arrangement of hepatic cords was disordered,and inflammatory cells infiltrated.In the ATPR group,the intercellu-lar space of liver and the structure of hepatic cords were restored,and the inflammatory cell infiltration was less.TEM showed that the damaged mitochondria and lipid droplet accumulation in the hepatocytes of mice in the model group were compared with that in the normal group,and the morphology and quantity of mitochondria and lipid droplet in the hepatocytes of mice in the ATPR group tended to be normal.Western blot showed that compared with the normal group,the expression of FUNDC1 protein in the liver tissues of mice in the model group increased,the expression of OPA1 protein decreased,the ratio of LC3B Ⅱ to LC3B Ⅰ decreased,the expression of P62 protein in-creased,the expression of Beclin1 and ATG5 protein decreased,and the above changes were reversed in the ATPR group.Conclusion ATPR alleviates acute liver injury induced by lipopolysaccharide in mice by promoting autoph-agy.
الملخص
Objective @#To investigate the effect of cysteine rich acidic secretory protein like protein 1 (SPARCL1) on atherosclerosis (AS) plaque formation .@*Methods @#A case control study design was used , 394 patients with con firmed AS were selected as the case group , and 394 healthy medical examiners matched for age and gender were se lected as the control group . The expression level of serum SPARCL1 was determined by enzyme linked immunosor bent assay; immunohistochemistry was used to assess the expression level and localization of SPARCL1 protein in the AS plaque region , and the expression of SPARCL1 protein was also detected in the neutrophils and monocytes of peripheral blood of AS patients and normal controls; SPARCL1 overexpressing and the recombinant adenoviral vec tors were constructed to inhibit SPARCL1 overexpression and expression , and the effects of SPARCL1 on cell mi gration were ob served in the cell scratch assay using mouse macrophage cells (J774A.1) as target cells .@*Results@#Serum SPARCL1 levels in the AS patient group were lower than those in the healthy group ( P < 0.05 ) ; high SPARCL1 expression was detected in AS plaques and was mainly expressed in the cytoplasm of foamy cells; SPARCL1 expression levels in peripheral blood neutrophils and monocytes were lower than those in normal controls in AS patients (P < 0.05) ; recombinant SPARCL1 overexpression and inhibition of expression of adenovirus was successfully constructed; the cell migration rate was decreased in J774A.1 cells that inhibited SPARCL1 expression and increased in J774A.1 cells that overexpressed SPARCL1 ( P < 0.05) .@*Conclusion @#SPARCL1 is highly expressed in foam cells at the site of AS lesions , which may result from compensatory recruitment of peripheral blood monocytes and neutrophils , and SPARCL1 may be involved as a protective factors for blood vessels in inhibiting the development of AS plaques .
الملخص
Objective @# Cas9-RNP biomimetic nanoparticles cas9-RNP@ MMs were prepared by encapsulating the Cas9 Ribonucleoprotein complex (RNP) using mouse macrophage membranes,with the aim of utilizing this biomimetic nanoparticle to deliver the Cas9-RNP complex for gene editing ,and further study the endocytosis of Cas9- RNP@ MMs and its gene editing effect in mouse macrophage RAW264. 7 in vitro ,providing evidence for the development oflow-toxicity biomimetic nanoparticle carriers that inhibit NLRP3 therapeutic targets.@*Methods @#The purified mouse macrophage membrane was mixed with the prepared cas9-RNP mixture,and after ultrasound,the CAS9- RNP@ MMS was obtained by liposome extrusion instrument ; The particle size of Cas9-RNP@ MMswas measured by nanoparticle tracking analysis,and the particle morphology of Cas9-RNP@ MMs was observed under transmission electron microscope.Laser confocal Fluorescence microscope imaging was used to analyze the endocytosis Cas9-RNP @ MMs.The Biocompatibility of Cas9-RNP@ MMs was measured by MTT assay.The expression of NLRP3 was detected by qPCR and Western blot to verify the knockdown effect of Cas9-RNP@ MMs on NLRP3 gene. @*Results@#The average particle diameter of Cas9-RNP@ MMs prepared from macrophages was about 216 nm.Under laser confocal fluorescence microscope,the Cas9-RNP@ MMs could be successfully endocysed by Raw246. 7 cell.MTT assay indicated that the Cas9-RNP@ MMs-treated mouse macrophage RAW246. 7 had good biocompatibility.qPCR and Western blot showed that two NLRP3-specific guide RNA were mediated by Cas9-RNP@ MMs,with good effect of knockdown NLRP3 gene expression.@*Conclusion@# Nano-scale vesicles Cas9-RNP@ MMs loaded with Cas9-RNP complexes were successfully prepared by biomimetic nanoparticles. Cas9-RNP@ MMs have good biocompatibility and can be efficiently endocytosed by RAW246. 7 cells.Cas9-RNP@ MMs containing NLRP3-specific sgRNA can specifically knock down NLRP3 gene expression.
الملخص
Objective @#To investigate the effect and mechanism of all-trans retinoic acid (ATRA) on lipopolysaccharide (LPS) -induced acute myocardial injury in C57BL/6 mice.@*Methods @#Male mice of C57BL/6 strain were randomly divided into normal group,model group,ATRA group,and ferrostatin-1 group.Mice in the ATRA group were injected intraperitoneally with ATRA 15mg / (kg · d) ,ferrostatin-1 group received ferrostatin-1 2 mg / ( kg · d) ,the normal group and the model group were given solvent.After one week of continuous administration,the model group,ATRA group ,and ferrostatin-1 group were intraperitoneally injected with LPS 6 mg / kg. All mice were sacrificed after 6 hours.The contents of malondialdehyde ( MDA) and glutathione ( GSH) in serum of mice were detected. qPCR was used to detect mRNA levels of interleukin-6 ( IL-6 ) and tumor necrosis factor-alpha (TNF-α) in heart tissue.Hematoxylin-eosin ( HE) staining was used to observe the changes of heart tissue in mice.Transmission electron microscopy (TEM) was used to observe the structure of mouse myocardial mitochondria.Western blot was used to detect the expression of ferroptosis markers glutathione peroxidase 4 ( GPX4) ,ferritin heavy chain 1 ( FTH1 ) ,Solute carrier family 7 member 11 ( SLC7A11 ) ,acyl-CoA synthetase long-chain family member 4 (ACSL4) and related regulatory proteins,Nuclear factor erythroid 2-related factor 2 ( NRF2 ) ,kelchlike ECH-associated protein 1 (KEAP1) . @*Results@#Compared with the normal group,the MDA content in the serum of the model group increased and the GSH content decreased,the above changes were reversed in the ATRA group as well as in the ferrostatin-1 group.Compared with normal group,the mRNA levels of IL-6 and TNF-α in the heart tissue of model group increased steeply,the above changes were relieved in the ATRA group and the ferrostatin-1 group.There was no significant difference in HE staining of myocardial tissue among the groups of mice. Compared with the normal group,myocardial mitochondria in the model group showed the phenomenon of cristaereduction or disappearance under TEM,while myocardial mitochondrial injury was alleviated in the ATRA group and the ferrostatin-1 group.Western blot showed that GPX4,FTH1,SLC7A11,and NRF2 expression were reduced in the myocardial tissue of mice in the model group compared with the normal group,ACSL4 and KEAP1 expression increased.The above changes were reversed in the ATRA group as well as in the ferrostatin-1 group.@*Conclusion@#ATRA alleviates lipopolysaccharide-induced acute myocardial injury in mice by inhibiting ferroptosis.
الملخص
Objective@#To solve the problems of low throughput of current cell migration research methods,which was difficult to establish a stable concentration gradient and observe cell migration behavior in real time,a six-channel array microfluidic chip was designed in this paper.@*Methods @#In this paper,a six-channel array microfluidic chip is designed.Firstly,multiphysics modeling and numerical simulation were performed using the finite element analysis software COMSOL Multiphysics 5.5 to analyze the flow behavior of the main pipeline of cell migration. Then,the throughput advantage of the device was verified by testing the chemotaxis response of healthy human neutrophils to different types of chemokine gradients in this microfluidic chip.Subsequently,by analyzing the migration rate of neutrophils in 6 patients with type II diabetes mellitus and 3 healthy people,the clinical applicability of the annular six-channel array microfluidic chip was further verified.Finally,the Pearson coefficient was used to analyze the correlation between neutrophil chemotaxis function and some physiological indicators in patients with diabetes. @*Results@#The concentration gradient data inside the pipeline simulated by the simulation software was compatible with the real-time fluorescence test data of the pipeline.The average migration rate of healthy human neutrophils was (0.21 ± 0.01 ) μm / s in 100 nmol / L interleukin-8 ( IL-8 ) environment and (0.22 ± 0.01 ) μm / s in 100 nmol / L N-Formyl-Met-Leu-Phe ( fMLP) environment. In the comparison of neutrophil migration experiments between healthy people and diabetic patients,the chemotaxis rate of neutrophils in healthy people was (0.19 ± 0.01) μm / s ,and the neutrophil chemotaxis rate in diabetic patients was (0. 15 ± 0. 02 ) μm / s. Correlation analysis showed that neutrophil migration rate in patients with type II diabetes mellitus was inversely correlated with glycated hemoglobin.@*Conclusion@#The high-throughput microfluidic chip proposed in this paper allowed rapid and selective detection of cell migration characteristics at the single-cell level,and it could be used as a new tool for cell migration research.
الملخص
AIM To study the effect of Vit E on the MLCK activity and expression in the liver of atherosclerosis model rabbits. METHODS The MLCK activity of rabbit liver was measured by the method of ?- 32P incorporated and its expression was detected by immunofluorescent. RESULTS The model of atherosclerosis was estabilished. After rabbits were fed with cholesterol for four weeks and twelve weeks, the activity of MLCK increased markedly, and there was significantly statistical difference compared with the normal control (P0.05). MLCK expression increased after the rabbits was fed with cholesterol for four weeks, and this increase became more obvious had been the rabbits was fed with cholesterol for twelve weeks. The expression decreased when vitamin E had been added into the cholesterol fed. CONCLUSION The pathology of liver may be associated with the increase of the activity of MLCK. Vit E may reduce MLCK activity and protect hepatocyte from injury.
الملخص
Aim To study the effect of melatonin on expression and activity of myosin light chain kinase in the artery wall of atherosclerotic rabbits.Methods The rabbit model of atherosclerosis was induced by a high-cholesterol diet.The blood lipid levels were assayed in the serum of each group.MLCK expression was detected by Western blot and immunohistochemical method.MLCK activity was measured by ?-32P-ATP incorporation into myosin light chain.Results The atherosclerosis model was established successfully.The levels of lipids decreased after MLT treatment.After fed with cholesterol for twelve weeks,the expression and activity of MLCK in the artery of atherosclerotic rabbits increased markedly,whereas there was no obvious difference in expression of MLCK in the artery of atherosclerotic rabbits fed with cholesterol and melatonin for twelve weeks compared with that of control.Conclusions It was suggest that high expression and activity of MLCK in the artery might be closely correlated with the development of atherosclerosis.Melatonin played an important role in inhibiting the development of atherosclerosis by decreasing the expression and activity of MLCK.