Recombinant chitinase-3-like protein 1 alleviates learning and memory impairments via M2 microglia polarization in postoperative cognitive dysfunction mice

Postoperative cognitive dysfunction is a seve re complication of the central nervous system that occurs after anesthesia and surgery,and has received attention for its high incidence and effect on the quality of life of patients.To date,there are no viable treatment options for postoperative cognitive dysfunction.The identification of postoperative cognitive dysfunction hub genes could provide new research directions and therapeutic targets for future research.To identify the signaling mechanisms contributing to postoperative cognitive dysfunction,we first conducted Gene Ontology and Kyoto Encyclopedia of Genes and Genomes pathway enrichment analyses of the Gene Expression Omnibus GSE95426 dataset,which consists of mRNAs and long non-coding RNAs differentially expressed in mouse hippocampus3 days after tibial fracture.The dataset was enriched in genes associated with the biological process"regulation of immune cells,"of which Chill was identified as a hub gene.Therefore,we investigated the contribution of chitinase-3-like protein 1 protein expression changes to postoperative cognitive dysfunction in the mouse model of tibial fractu re surgery.Mice were intraperitoneally injected with vehicle or recombinant chitinase-3-like protein 124 hours post-surgery,and the injection groups were compared with untreated control mice for learning and memory capacities using the Y-maze and fear conditioning tests.In addition,protein expression levels of proinflammatory factors(interleukin-1βand inducible nitric oxide synthase),M2-type macrophage markers(CD206 and arginase-1),and cognition-related proteins(brain-derived neurotropic factor and phosphorylated NMDA receptor subunit NR2B)were measured in hippocampus by western blotting.Treatment with recombinant chitinase-3-like protein 1 prevented surgery-induced cognitive impairment,downregulated interleukin-1βand nducible nitric oxide synthase expression,and upregulated CD206,arginase-1,pNR2B,and brain-derived neurotropic factor expression compared with vehicle treatment.Intraperitoneal administration of the specific ERK inhibitor PD98059 diminished the effects of recombinant chitinase-3-like protein 1.Collectively,our findings suggest that recombinant chitinase-3-like protein 1 ameliorates surgery-induced cognitive decline by attenuating neuroinflammation via M2 microglial polarization in the hippocampus.Therefore,recombinant chitinase-3-like protein1 may have therapeutic potential fo r postoperative cognitive dysfunction.

Obtaining High Pest_resistant Transgenic Upland Cotton Cultivars Carrying cry1Ac3 Gene Driven by Chimeric OM Promoter

Hypocotyl segments from aseptic seedlings of two important cultivars of upland cotton ( Gossypium hirsutum L.) in Northwest China, 'Xinluzao_1', 'Jinmian_7', 'Jinmian_12' and 'Jihe_321' were transformed respectively by two efficient plant expression plasmids pBinMoBc and pBinoBc via Agrobacterium tumefaciens . In pBinMoBc, cry 1Ac3 gene, which encodes the Bt toxin, is under the control of chimeric OM promoter. In pBinoBc, it is under control of CaMV 35S promoter. After co_cultivation with Agrobacterium tumefimpfaciens LBA4404 (containing pBinMoBc or pBinoBc), kanamycin_resistant selection, somatic embryos were induced and regenerated plants were obtained. Then the regenerated plantlets were grafted to untransformed stocks in greenhouse to produce descendants. The integration of cry 1Ac3 gene and its expression in T 2 generation of transgenic cotton plants were confirmed by Southern hybridization and Western blotting. The analyses of insect bioassay indicated that the transgenic plants of both constructions have significant resistance to the larvae of cotton bollworm ( Heliothis armigera ) and that cry 1Ac3 gene driven by chimeric OM promoter could endue T 2 generation cotton with high pest_resistant ability, implicating that it has a profound application in genetic engineering to breed new pest_resistant cotton varieties.

Heat-inducible SlWRKY3 confers thermotolerance by activating the SlGRXS1 gene cluster in tomato

High temperature stress is one of the major environmental factors that affect the growth and development of plants. Although WRKY transcription factors play a critical role in stress responses, there are few studies on the regulation of heat stress by WRKY transcription factors,especially in tomato. Here, we identified a group I WRKY transcription factor, SlWRKY3, involved in thermotolerance in tomato. First, SlWRKY3 was induced and upregulated under heat stress. Accordingly, overexpression of SlWRKY3 led to an increase, whereas knock-out of SlWRKY3 resulted in decreased tolerance to heat stress. Overexpression of SlWRKY3 accumulated less reactive oxygen species(ROS), whereas knock-out of SlWRKY3 accumulated more ROS under heat stress. This indicated that SlWRKY3 positively regulates heat stress in tomato. In addition,SlWRKY3 activated the expression of a range of abiotic stress-responsive genes involved in ROS scavenging, such as a SlGRXS1 gene cluster.Further analysis showed that SlWRKY3 can bind to the promoters of the SlGRXS1 gene cluster and activate their expression. Collectively, these results imply that SlWRKY3 is a positive regulator of thermotolerance through direct binding to the promoters of the SlGRXS1 gene cluster and activating their expression and ROS scavenging.

A novel splice site mutation of CRYBA3/A 1 gene associated with congenital cataract in a Chinese family

AIM： To identify the disease-causing mutation responsible for the presence of congenital cataract in a Chinese family. METHODS： The study recruited a four-generation Chinese pedigree affected by autosomal dominant congenital cataract （ADCC）. Family history and the history of cataract extraction were recorded. Blood samples were collected from individuals for DNA extraction. Direct sequencing of congenital cataract-associated genes was performed. Single-strand conformational polymorphism and bioinformatic analysis were conducted to further study the mutation. RESULTS： Direct sequencing revealed a novel splice site mutation of c.30-2 A〉G in the CRYBA3/A1 gene. The mutation co-segregated within all affected individuals in the family and was not found in unaffected members or 100 unrelated normal controls. These results were further confirmed by single-strand conformational polymorphism and bioinformatic analysis using the Human Splicing Finder and MaxEnt online software and Annovar computer software. CONCLUSION： c,30-2 A〉G mutation of CRYBA3/A1 gene is a novel mutation and broadens the genetic spectrum of ADCC, KEYWORDS： splice site mutation; congenital cataract; CRYBA3/A1 gene

慢性肾小球肾炎患者血清CHI3L1、HSP60表达水平及其临床意义

目的探讨慢性肾小球肾炎(CGN)患者血清壳多糖酶3样蛋白1(CHI3L1)、热休克蛋白60(HSP60)表达水平及其临床意义。方法选择97例CGN患者为CGN组,另选取体检健康者120例为健康组。对CGN组随访12个月,根据预后分为预后良好组(n=79)和预后不良组(n=18)。采用酶联免疫吸附法检测血清CHI3L1、HSP60水平,采用全自动生化分析仪检测肾功能指标,分析CHI3L1、HSP60与肾功能指标的相关性。采用ROC分析CHI3L1、HSP60对CGN患者预后的预测价值。结果CGN组血清CHI3L1、HSP60高于健康组(P<0.05)。CGN组、预后不良组血尿素氮、血肌酐、血尿酸分别高于健康组、预后良好组(P<0.05)。Pearson相关分析结果显示,血清CHI3L1、HSP60与血尿素氮、血肌酐、血尿酸均呈正相关(P<0.001)。血清CHI3L1、HSP60联合预测CGN患者预后的效能最高(P<0.001)。结论CGN患者血清CHI3L1、HSP60水平升高,其可作为预测患者预后的潜在生物标志物。

血清CHI3L1水平与肝脏疾病之间的关系

目的 通过壳多糖酶3样蛋白1(chitinase 3-like protein 1,CHI3L1)在慢性乙型肝炎(chronic hepatitis B,CHB)、自身免疫性肝病(autoimmune liver disease, AILD)、肝硬化(liver cirrhosis, LC)、肝癌(hepatocellular carcinoma, HC)中的水平,为临床监测肝脏疾病进展提供依据。方法 选取菏泽市立医院2022年6月至2023年12月健康体检者60例、慢性乙型肝炎患者60例、自身免疫性肝病患者60例、肝硬化患者60例、肝癌患者60例作为研究对象,应用酶联免疫吸附(ELISA)法检测所有研究对象血清中CHI3L1表达水平;应用流式细胞检测细胞因子表达水平;生化分析仪检测生化指标水平。结果 CHI3L1水平,健康体检组(47.00±20.50ng/mL)<CHB组(91.75±35.58ng/mL)<AILD组(128.30±41.92ng/mL)<LC组(131.29±46.52ng/mL)<HC组(154.07±59.92ng/mL)。以健康体检组为对照,CHI3L1诊断LC的ROC曲线显示,AUC为0.965;CHI3L1诊断HC的ROC曲线显示AUC为0.974。以慢性乙型肝炎组为对照,CHI3L1诊断肝硬化的值AUC为0.749(P<0.001),CHI3L1+AST诊断肝硬化AUC值为0.845(P<0.001),优于CHI3L1检测;以慢性乙型肝炎组为对照,AFP诊断HC的AUC为0.783,CHI3L1诊断HC的AUC为0.800(P<0.001);CHI3L1+AFP诊断HC的AUC为0.891,CHI3L1+AST+IL-17+IL-6诊断肝癌的AUC为0.937(P<0.001),优于CHI3L1和AFP检测。结论 血清CHI3L1表达水平在肝癌组中最高,慢性乙型肝炎组最低,血清CHI3L1表达水平随疾病进展升高;血清CHI3L1可作为辅助诊断肝硬化和肝癌的无创指标;血清CHI3L1、AST、IL-6、IL-17、IL-8、IFN-γ联合检测能够提高对肝硬化和肝癌的诊断。

2型糖尿病患者血清SFRP-4和CHI3L1水平对糖尿病视网膜病变的评估价值

目的:探讨2型糖尿病(DM)患者血清分泌型卷曲蛋白-4(SFRP-4)、壳多糖3样蛋白1(CHI3L1)水平与糖尿病视网膜病变(DR)的相关性。方法:前瞻性研究。选取2018-10/2023-10本院收治的DR患者103例为DR组,其中DR早期39例,DR中期42例,DR晚期22例;选取单纯2型糖尿病患者98例为DM组,同期选取健康体检者101例为对照组。收集各组受试者基线资料及临床指标。采用酶联免疫吸附(ELISA)法检测血清SFRP-4、CHI3L1水平。结果:DR组患者血清SFRP-4、CHI3L1水平及TG、LDL-C、HbA1C、FPG、HOMA-IR均高于DM组和对照组(均P<0.05);DM组患者血清SFRP-4、CHI3L1水平及TG、LDL-C、HbA1C、FPG、HOMA-IR均高于对照组(均P<0.05)。DR晚期患者病程、TG、LDL-C、HbA1C、FPG、HOMA-IR、SFRP-4、CHI3L1均高于DR中期、DR早期(均P<0.05)。DR患者血清SFRP-4、CHI3L1水平与病程、TG、LDL-C、HbA1C、FPG、HOMA-IR、DR分期均呈正相关(均P<0.05)。血清SFRP-4、CHI3L1及联合诊断DR的曲线下面积(AUC)分别为0.809、0.801、0.898。血清SFRP-4、CHI3L1水平是影响DR发生的危险因素(P<0.05)。结论:血清SFRP-4、CHI3L1水平与2型糖尿病患者DR关系密切,二者水平升高提示患者发生DR的风险较高。

多层螺旋CT联合血清CHI3L1、ANGPTL2对胆囊癌的诊断价值

胆囊癌是胆道系统恶性肿瘤,患者会出现黄疸、腹痛等症状,还会出现胆囊炎和胆囊穿孔等[1,2]。胆囊癌在早期会对邻近周围器官肝脏进行侵犯,不适合进行根治性手术,而且患者易产生化疗耐药性,导致预后不良[3,4]。因此在早期诊断胆囊癌尤为重要。多层螺旋CT(multi-slice spiral CT,MSCT)能提高早期诊断恶性肿瘤准确率,但也在影像学图像判断上存在局限[5]。壳多糖酶3样蛋白1(chitosan enzyme 3-like protein 1,CHI3L1)可参与机体炎症以及血管形成[6]。CHI3L1在多种癌症中呈现高表达[7]。血管生成素样蛋白2(angiopoietin-like protein 2,ANGPTL2)作为癌症治疗的靶点,可参与乳腺癌进展[8]。目前关于MSCT联合血清CHI3L1、ANGPTL2在胆囊癌中的研究鲜有报道,因此,本研究旨在探讨MSCT联合血清CHI3L1、ANGPTL2对胆囊癌的诊断价值。

Analysis of the autophagy gene expression profile of pancreatic cancer based on autophagy-related protein microtubule-associated protein 1A/1B-light chain 3

BACKGROUND Pancreatic cancer is a highly invasive malignant tumor. Expression levels of the autophagy-related protein microtubule-associated protein 1 A/1 B-light chain 3(LC3) and perineural invasion(PNI) are closely related to its occurrence and development. Our previous results showed that the high expression of LC3 was positively correlated with PNI in the patients with pancreatic cancer. In this study, we further searched for differential genes involved in autophagy of pancreatic cancer by gene expression profiling and analyzed their biological functions in pancreatic cancer, which provides a theoretical basis for elucidating the pathophysiological mechanism of autophagy in pancreatic cancer and PNI.AIM To identify differentially expressed genes involved in pancreatic cancer autophagy and explore the pathogenesis at the molecular level.METHODS Two sets of gene expression profiles of pancreatic cancer/normal tissue(GSE16515 and GSE15471) were collected from the Gene Expression Omnibus.Significance analysis of microarrays algorithm was used to screen differentially expressed genes related to pancreatic cancer. Gene Ontology(GO) analysis and Kyoto Encyclopedia of Genes and Genomes(KEGG) pathway analysis were used to analyze the functional enrichment of the differentially expressed genes. Protein interaction data containing only differentially expressed genes was downloaded from String database and screened. Module mining was carried out by Cytoscape software and ClusterOne plug-in. The interaction relationship between the modules was analyzed and the pivot nodes between the functional modules were determined according to the information of the functional modules and the data of reliable protein interaction network.RESULTS Based on the above two data sets of pancreatic tissue total gene expression, 6098 and 12928 differentially expressed genes were obtained by analysis of genes with higher phenotypic correlation. After extracting the intersection of the two differential gene sets, 4870 genes were determined. GO analysis showed that 14 significant functional items including negative regulation of protein ubiquitination were closely related to autophagy. A total of 986 differentially expressed genes were enriched in these functional items. After eliminating the autophagy related genes of human cancer cells which had been defined, 347 differentially expressed genes were obtained. KEGG pathway analysis showed that the pathways hsa04144 and hsa04020 were related to autophagy. In addition,65 clustering modules were screened after the protein interaction network was constructed based on String database, and module 32 contains the LC3 gene,which interacts with multiple autophagy-related genes. Moreover, ubiquitin C acts as a pivot node in functional modules to connect multiple modules related to pancreatic cancer and autophagy.CONCLUSION Three hundred and forty-seven genes associated with autophagy in human pancreatic cancer were concentrated, and a key gene ubiquitin C which is closely related to the occurrence of PNI was determined, suggesting that LC3 may influence the PNI and prognosis of pancreatic cancer through ubiquitin C.

Sequence Variations in the Bovine IGF-I and IGFBP3 Genes and Their Association with Growth and Development Traits in Chinese Beef Cattle

The objective of this study was to determine the genotype effects of the bovine insulin-like growth factor Ⅰ （IGF-Ⅰ） and its binding protein 3 （IGFBP3） genes on growth and development traits in beef cows, including 130 Chinese Simmental, 42 Nanyang, and 47 Luxi Yellow cattle. Sequence variations in the bovine IGF-Ⅰ and IGFBP3 genes were investigated by single strand conformation polymorphism （SSCP）. SSCPs were detected in 6 fragments, which is the 5＇-flanking region, the 2nd exon, the 5th exon, and the 5th intron of the IGF-1 gene, and the 2nd exon, the 3rd exon of the 1GFBP3 gene. Two polymorphisms, an A-to-G transition in the 2rid exon of the IGF-Ⅰ gene and a T-to-C transition in the 2rid exon of IGFBP3 gene were detected in 3 breeds. The allele frequencies of 2 polymorphisms were 0.0411 （A）, 0.9589 （B）, and 0.7237 （A）, 0.2763 （B）, respectively. These 2 loci were analyzed to associate with body weight, height at withers, body length, heart girth, rump width, and beef production index （BPI） at 0, 6, 12, 24, and 36-month old. The IGFBP3 locus was shown to be associated with rump width, heart girth at 24-month and 36-month. Animals with BB genotype had higher rump width （24.86 ± 0.47） cm at 24-month and （27.50 ± 0.63） em at 36-month. The heart girth was highest for the individuals with BB genotype （171.33 ± 1.84） cm and higher than those with AB genotype （166.68 ± 1.13） cm （P〈 0.05） at 36-month.

Transferring a Gene Expression Cassette Lacking the Vector Backbone Sequences of the 1Ax1 High Molecular Weight Glutenin Subunit into Two Chinese Hexaploid Wheat Genotypes

1Ax1 high molecular weight glutenin subunit （HMW-GS） gene expression cassette （GEC） lacking vector backbone sequences together with selectable marker Bar GEC were co-transformed into Chinese hexaploid cultivars Een 1 and Emai 12 to test the feasibility and the efficiency of explant regeneration, transformation frequency and transgene expression comparing with whole vector transformation by the approaches of plasmid extraction and excision, immature embryo isolation, particle co-bombardment, tissue culture, DNA extraction, PCR amplification, southern hybridization, leaf-painting test and SDS-PAGE etc. No significant difference was shown in tissue culture response of the proportion of embryogenic calli, somatic embryogenesis and regeneration frequency between GEC and whole plasmid bombarded embryos, but both regenerated less well than non-bombarded control. Total 56 plantlets that survived PPT selection had insertion of at least the Bar gene, 18 were from the GEC treatment and 38 from the whole plasmid treatment, the escape ratio averaged 0.23. Six independent transplants f230 - f235 with GEC transformation from genotype Emai 12 presented clear PCR amplification bands of Bar and 1Ax1 gene. The transformation and co-transformation frequency were 3.51 and 100% respectively. PCR amplification using a primer-pair specific for ampicillin resistant gene indicated the existence of Amp^R gene in whole vectors but the removal in GECs and transplants. Southern blot of total DNA and PCR products from transgenic plants of 1Ax1 GEC confirmed the integration of the transgene 1Ax1 and the absence of the EcoR Ⅰ recognition site at both ends of the 1Ax1 GEC when integrated. SDS-PAGE showed the expression of 1Ax1 GEC and un-expression of whole plasmid. The length of integrated fragment, the proportion of the gene of interest （GOI） and the selectable marker （MG）, bombardment pressure and genotypes are vital for the expression of a transformed GEC.

EMP-1 Promotes Tumorigenesis of NSCLC through PI3K/AKT Pathway

This study examined the role of EMP-1 in tumorigenesis of non-small cell lung carcinoma (NSCLC) and the possible mechanism. Specimens were collected from 28 patients with benign lung diseases and 28 with NSCLC, and immunohis to chemically detected to evaluate the correlation of EMP-1 expression to the clinical features of NSCLC. Recombinant adenovirus was constructed to over-express EMP-1 and then infect PC9 cells. Cell proliferation was measured by Ki67 staining. Western blotting was performed to examine the effect of EMP-1 on the PI3K/AKT signaling. Moreover, tumor xeno-grafts were established by subcutaneous injection of PC9 cell suspension (about 5×107/mL in 100 μL of PBS) into the right hind limbs of athymic nude mice. The results showed EMP-1 was significantly up-regulated in NSCLC patients as compared with those with benign lung diseases. Over-expression of EMP-1 promoted proliferation of PC9 cells, which coincided with the activation of the PI3K/AKT pathway. EMP-1 promoted the growth of xenografts of PC9 cells in athymic nude mice. It was concluded that EMP-1 expression may contribute to the development and progress of NSCLC by activating PI3K/AKT pathway.

Development of Hybrid Rice Variety FY7206 with Blast Resistance Gene Pid3 and Cold Tolerance Gene Ctb1

Hybrid rice Fanyou 7206（FY7206）, derived from the cross between a sterile line Fanyuan A and a restorer line Fuhui 7206, was bred by the Rice Research Institute, Fujian Academy of Agricultural Sciences, China. FY7206 was characterized by moderate blast resistance, cold tolerance, as well as wide adaptability, and high yields. The blast resistance results indicated that the frequencies of blast races in race B, race C and the total resistance frequency for FY7206 were 95.5%, 100.0% and 97.2%, respectively. The disease resistance results showed that the leaf blast grade for FY7206 was level 1 and panicle blast was level 5. The indoor spray results indicated that FY7206 was resistant to 11 isolates of Magnorpathe oryzae. The blast resistance of FY7206 might be derived from the high expression of blast resistance gene Pid3. The results for simulated cold resistance in an artificial climate chamber indicated that the cold tolerance for FY7206 was moderate at the booting and flowering stages. The cold tolerance results also indicated that FY7206 could be tolerant to temperatures as low as 10 °C at the seedling stage. The q RT-PCR results showed that the expression of cold tolerance gene Ctb1 in FY7206 was relatively high. These results suggested that FY7206 is a hybrid indica rice variety with good comprehensive characteristics, including blast resistance and cold tolerance.

Expression of <i>T4HR1</i>, a 1,3,6,8-Tetrahydroxynaphthalene Reductase Gene Involved in Melanin Biosynthesis, Is Enhanced by Near-Ultraviolet Irradiation in <i>Bipolaris oryzae</i>

Bipolaris oryzae is the causal agent of brown spot disease in rice and produces the dark pigment melanin. We isolated and characterized T4HR1 gene encoding 1,3,6,8-tetrahydroxynaphthalene (1,3,6,8-THN) reductase, which converted 1,3,6,8-THN to scytalone in the melanin biosynthesis from B. oryzae. A sequence analysis showed that the T4HR1 gene encoded a putative protein of 268 amino acids showing 50% - 99% sequence identity to other fungal 1,3,6,8-THN reductases. Targeted disruption of the T4HR1 gene showed a different phenotype of mycelial color due to an accumulation of shunt products compared to those of wild-type on PDA plates using tricyclazole as a melanin biosynthesis inhibitor. A quantitative real-time PCR analysis showed that the expression of T4HR1 transcripts was enhanced by near-ultraviolet (NUV) irradiation and regulated by transcriptional factor BMR1, similar to three other melanin biosynthesis genes (polyketide synthase gene [PKS1], scytalone dehydratase gene [SCD1], and 1,3,8-THN reductase gene [THR1]) in the melanin biosynthesis of B. oryzae. These results suggested that common transcriptional mechanisms could regulate the enhanced gene expression of these melanin biosynthesis genes by NUV irradiation in B. oryzae.

Cloning and Bioinformatics Analysis of Rosa rugosa β-1,3-Glucanase Gene (RrGlu)

In order to reveal which role the callose played in R. rugosa pollination incompatibility, the full-length cDNA sequence of β-1,3-glucanase gene was cloned for the first time from the stylus of Rosa rugosa “Tanghong” with RT-PCR and RACE methods and named as RrGlu. The full-length cDNA is 1380 bp with an open reading frame of 1041 bp, encoding 346 amino acids. The derived protein has a molecular weight of 37.85 kD, a calculated pI of 9.12, a pfam00332 conserved domain at position 36 - 345, and belongs to glycosyl hydrolase family 17. The derived protein is a hydrophilic protein secreted into the vacuole. There is a signal peptide cleavage site at position 34 - 35, a transmembrane domain at position 13 - 32, six Ser phosphorylation sites, three Thr phosphorylation sites, three Tyr phosphorylation sites, one N-glycosylation site, and five O-glycosylation sites. There are 31.50% α-helixes, 30.92% random coil, 25.14% extended peptide chain, and 12.43% β-corner structure. This protein and the Glu protein from eight other species, including Prunus persica, share a sequence homology of greater than 72%;all of the proteins contain a pfam00332 conserved domain and a β-1,3-glucanase active center sequence (LIVM)-X-(LIVMFYW)3-(STAG)-E-(ST)-G-W-P-(ST)-X-G. Furthermore, their phylogenetic relationships are consistent with their traditional classifications. These results were meaningful to reveal the molecular mechanism of R. rugosa pollination incompatibility and improve the theory and techniques of breeding ornamental R. rugosa.

牙周病患者基础治疗前后唾液及血浆中CHI3L1、CHIT1水平的变化

目的:探讨牙周病患者牙周基础治疗前后其唾液、血浆中几丁质酶3样蛋白l(CHI3L1)、几丁质酶1(CHIT1)的水平变化及临床意义。方法:通过酶联免疫吸附法ELISA检测27例慢性牙周炎患者、17例慢性牙龈炎患者牙周基础治疗前后的唾液及血浆中CHI3L1、CHIT1的表达水平,并与20例健康对照者的样本进行比较。结果:CHI3L1在慢性牙周炎患者唾液中的表达水平显著高于对照组,且在牙周基础治疗后其表达水平显著降低,与治疗前相比差异具有统计学意义(P<0.05);慢性牙龈炎患者唾液中的CHI3L1表达水平与对照组及治疗后相比,差异无统计学意义(P>0.05);各组唾液及血浆中的CHIT1表达水平两两相比,差异均无统计学意义(P>0.05)。结论:CHI3L1可作为一种新的评估慢性牙周炎病变进展程度的生物学标记物。

CHI3L1通过激活TGF-β信号通路促进肝细胞肝癌进展及分子机制

目的观察CHI3L1对肝细胞肝癌Huh7增殖、迁移、侵袭的影响及其分子机制。方法通过脂质体转染,观察CHI3L1对Huh7增殖、迁移、侵袭的影响。通过染色质免疫共沉淀、Western blot观察CHI3L1对TGF-β信号通路的作用机制。结果转染CHI3L1后,Huh7细胞增殖率显著高于空载组及空白对照组,差异有统计学意义(P<0.05)。转染CHI3L1后,迁移、侵袭至下层细胞数均显著多于空载组、空白对照组,差异有统计学意义(P<0.05)。转染CHI3L1后,TGF-β刺激后形成的Smad2/3/4复合物增加,CHI3L1促进TGF-β诱导下Smads复合物的形成。转染CHI3L1后的Huh7细胞对TGF-β刺激上调p53非依赖的细胞周期抑制因子p21、p15,下调c-myc,抑制Rb磷酸化,上调NOX4;TGF-β抑制剂LY364947可抑制此诱导效应。结论CHI3L1可促进肝细胞肝癌增殖、迁移、侵袭,这种作用可能通过激活TGF-β信号通路实现。

血清CHI3L1、CGRP、IL-23在慢性牙周炎患者中的表达及在病情、疗效评价中的作用探讨

目的:探讨血清几丁质酶3样蛋白1(CHI3L1)、降钙素基因相关肽(CGRP)、白细胞介素-23(IL-23)在慢性牙周炎(CP)患者血清中的表达及在病情、疗效评价中的作用。方法:纳入106例CP患者为病例组,106例健康体检者为健康对照组。ELISA检测对比2组血清CHI3L1、CGRP、IL-23水平、病例组不同病情程度、不同疗效患者血清CHI3L1、CGRP、IL-23水平,用Spearman相关分析血清CHI3L1、CGRP、IL-23水平与CP患者病情、疗效的相关性。结果:病例组血清CHI3L1、IL-23水平高于健康对照组(P<0.05),CGRP水平低于健康对照组(P<0.05);病例组病情程度为中重度患者血清CHI3L1、IL-23水平高于轻度患者(P<0.05),血清CGRP水平低于轻度患者(P<0.05);病例组疗效较差患者血清CHI3L1、IL-23水平高于疗效良好患者(P<0.05),CGRP水平低于疗效良好患者(P<0.05);血清CHI3L1、IL-23水平与患者病情程度呈正相关(P<0.05),与疗效呈负相关(P<0.05);血清CGRP水平与CP患者病情程度呈负相关(P<0.05),与患者疗效呈正相关(P<0.05)。结论:血清CHI3L1、IL-23在CP患者中呈高表达,血清CGRP呈低表达,且其表达与患者病情、疗效密切相关。

跑台运动对肥胖小鼠骨骼肌CHI3L1表达的影响及其机制

目的:观察跑台运动对高脂饮食诱导的肥胖小鼠骨骼肌几丁质酶-3样蛋白-1(CHI3L1)表达的影响及机制探讨。方法:5周龄健康雄性C57BL/6小鼠随机分成对照组和高脂喂养组,分别进行普通饲料和高脂饲料喂养,8周后筛选肥胖小鼠16只,随机分为高脂安静组和高脂运动组。跑台训练持续8周,每周5次,每次60分钟,跑速25米/分钟。测定小鼠体重,免疫组化法观察比目鱼肌和腓肠肌CHI3L1的蛋白表达水平,real-time PCR方法分别测定比目鱼肌和腓肠肌CHI3L1、TNF-α和IL-6的m RNA表达。结果:与对照组相比,高脂饮食喂养小鼠体重显著增加(P<0.01);比目鱼肌和腓肠肌CHI3L1的m RNA表达均显著上调(P<0.01和P<0.001),腓肠肌中CHI3L1的蛋白表达显著增加,比目鱼肌中CHI3L1的蛋白水平没有显著改变;腓肠肌TNF-α和IL-6 m RNA表达均显著上调(P<0.001和P<0.01),比目鱼肌中TNF-α和IL-6 m RNA表达有上调趋势,但无显著差异。与单纯高脂饮食组小鼠相比,8周跑台运动小鼠体重显著降低(P<0.01);比目鱼肌和腓肠肌CHI3L1 m RNA表达显著下降(P<0.001),CHI3L1蛋白表达均显著减少;腓肠肌TNF-α和IL-6 m RNA表达均显著下调(P<0.001和P<0.01),但比目鱼肌TNF-α和IL-6 m RNA表达无显著变化。结论:跑台运动能显著减少肥胖小鼠比目鱼肌和腓肠肌CHI3L1的表达,显著下调腓肠肌促炎因子TNF-α和IL-6的表达,提示运动通过减轻肥胖时骨骼肌炎症间接地调节骨骼肌CHI3L1表达。

Combinatorial Effects of SDF-1 and CCL3L1 Gene Variants and Susceptibility to HIV-1/AIDS in Indian Population

HIV-1 infection requires the expression of CD4＋ molecules in colligation with C-C chemokine receptor type 5 （CCR5） and C-X-C chemokine receptor type 4 （CXCR4） as the major coreceptors. The role of SNP in 3＇ untranslated region ofSDF-1 （SDF1-3 ＇A） and low copy number （CN） of the CCL3L1 gene is reported to confer increased resistance to HIV-1 infection. The aim of the present study was to analyze the combinatorial effect of both the variations in protection towards HIV-1 infection in Indian population. The combinatorial effect of genetic variation in terms of SNP in SDF-1 gene and CCL3L1 CN was investigated in 105 healthy individuals and 78 HIV-I patients. Genotyping of SDF-1 was performed by RFLP-PCR and CCL3L1 by real-time PCR using TaqMan chemistry. The genotype frequency distribution of SDF-1 was found to be （SDF-1/SDF-I： 65.4%, SDF-1/SDF1-3＇A： 29.5% and SDFI-3＇A/SDF1-3＇A- 5.1%） in HIV patients as compared to （SDF-1/SDF-I： 64.8%, SDF-1/SDF1-3＇A： 30.5% and SDF1-3 ＇A/SDF1-3 ＇A： 4.7%） in healthy individuals, whereas a range of 1 to 6 copies per diploid genome was observed for CCL3L1 gene.