牙本质涎磷蛋白、Ⅰ型胶原蛋白在vps4b基因敲除鼠磨牙牙胚发育中的时空表达

目的研究vps4b基因突变对牙齿发育相关蛋白——牙本质涎磷蛋白(DSPP)和Ⅰ型胶原蛋白(COL-Ⅰ)表达的影响。方法取胚胎E13.5 d、E14.5 d、E16.5 d的胎鼠头部及出生后P2.5 d、P7 d的幼鼠下颌骨组织,石蜡包埋后获取第一磨牙牙胚组织切片,采用免疫组织化学染色法检测野生型小鼠和vps4b基因敲除小鼠牙胚中DSPP、COL-Ⅰ的表达。结果野生鼠蕾状期和帽状期DSPP、COL-Ⅰ均未表达;钟状期DSPP在内釉上皮和牙乳头中有表达,COL-Ⅰ表达于牙乳头和牙囊;分泌期和矿化期DSPP、COL-Ⅰ在成釉细胞、成牙本质细胞、牙囊内均有表达,COL-Ⅰ在牙乳头内亦可见表达。小鼠vps4b基因敲除后,DSPP在钟状期牙乳头和分泌期牙乳头及牙囊内未见表达,COL-Ⅰ在钟状期及矿化期表达部位与野生型小鼠一致,分泌期在牙乳头的表达发生改变。结论 vps4b基因在牙胚发育中发挥重要作用;DSPP、COL-Ⅰ的表达可能受vps4b基因的调控,并与vps4b共同调节牙齿牙本质的发育。

Vps4b基因敲除鼠上皮根鞘中细胞角蛋白14和增殖细胞核抗原的表达

目的研究Vps4b基因突变对上皮根鞘(HERS)中细胞角蛋白14(CK14)和增殖细胞核抗原(PCNA)表达的影响。方法取出生后(P)5、9、11、15、19d的小鼠的双侧下颌组织,石蜡包埋后获得下颌第一磨牙组织切片,通过免疫组织化学方法比较CK14和PCNA在正常小鼠与Vps4b基因敲除小鼠HERS中的表达情况。结果正常小鼠P5d开始形成HERS,PCNA在HERS细胞中强阳性表达;P9d,HERS结构连续,PCNA在HERS细胞中阳性表达;P11d,一小部分HERS开始断裂,PCNA在HERS细胞中弱阳性表达;P15d,HERS继续断裂,PCNA在牙根表面HERS细胞中弱阳性表达;P19d,牙根达到生理长度,PCNA仅在牙根末端HERS细胞中阳性表达。基因敲除小鼠与正常小鼠相比,P5d同样形成HERS结构,然而其断裂在P9d就开始出现,P19d牙根表面仅存少量HERS碎片,根尖发育不成熟,PCNA表达强度下降。结论Vps4b基因突变可能通过改变HERS中CK14和PCNA的表达,从而导致牙根发育异常。

液泡分选蛋白4B在小鼠牙胚发育的时空表达

目的:研究液泡分选蛋白4B(vacuolar protein sorting 4B,VPS4B)在小鼠磨牙发育不同时期的表达。方法:取胚胎13.5、14.5、16.5 d的胎鼠头部及出生后2.5、7 d的幼鼠下颌骨组织,石蜡包埋后获取第一磨牙牙胚组织切片,通过组织化学染色确定各组牙胚的发育时期,免疫组织化学法检测牙胚中VPS4B的表达分布。结果:胚胎13.5、14.5、16.5 d小鼠第一磨牙牙胚分别处于蕾状期、帽状期、钟状早期,出生后2.5、7 d分别处于分泌期和矿化期;VPS4B表达于小鼠磨牙发育的整个过程,并在构成牙胚的多种细胞中有不同程度的表达。随发育的进行,成釉细胞和成牙本质细胞中VPS4B呈强阳性持续表达,而牙囊细胞表达逐渐减弱。结论:VPS4B表达于正常小鼠牙胚发育过程中且随发育进行表达发生改变,VPS4B可能参与牙胚的正常发育。

Cytoplasmic YAP1-mediated ESCRT-III assembly promotes autophagic cell death and is ubiquitinated by NEDD4L in breast cancer

Background:Nuclear Yes1-associated transcriptional regulator(YAP1)promotes tumor progression.However,the function of cytoplasmic YAP1 in breast cancer cells and its impact on the survival of breast cancer patients remain unclear.Our research aimed to explore the biological function of cytoplasmic YAP1 in breast cancer cells and the possibility of cytoplasmic YAP1 as a predictive marker of breast cancer survival.Methods:We constructed cell mutant models,including NLS-YAP15SA(nuclear localized),YAP1S94A(incapable of binding to the TEA domain transcription factor family)and YAP1S127D(cytoplasmic localized),and used Cell Counting Kit-8(CCK-8)assays,5-ethynyl-2’-deoxyuridine(EdU)incorporation assays,and Western blotting(WB)analysis to detect cell proliferation and apoptosis.The specific mechanism of cytoplasmic YAP1-mediated endosomal sorting complexes required for transport III(ESCRT-III)assembly was studied by co-immunoprecipitation,immunofluorescence staining,and WB analysis.Epigallocatechin gallate(EGCG)was used to simulate YAP1 retention in the cytoplasm in in vitro and in vivo experiments to study the function of cytoplasmic YAP1.YAP1 binding to NEDD4-like E3 ubiquitin protein ligase(NEDD4L)was identified using mass spectrometry and was verified in vitro.Breast tissue microarrays were used to analyze the relationship between cytoplasmic YAP1 expression and the survival of breast cancer patients.Results:YAP1 was mainly expressed in the cytoplasm in breast cancer cells.Cytoplasmic YAP1 promoted autophagic death of breast cancer cells.Cytoplasmic YAP1 bound to the ESCRT-III complex subunits charged multivesicular body protein 2B(CHMP2B)and vacuolar protein sorting 4 homolog B(VPS4B),promoting assembly of CHMP2B-VPS4B and activating autophagosome formation.EGCG retained YAP1 in the cytoplasm,promoting the assembly of CHMP2B-VPS4B to promote autophagic death of breast cancer cells.YAP1 bound to NEDD4L,and NEDD4L mediated ubiquitination and degradation of YAP1.Breast tissue microarrays revealed that high levels of cytoplasmic YAP1 were beneficial to the survival of breast cancer patients.Conclusions:Cytoplasmic YAP1 mediated autophagic death of breast cancer cells by promoting assembly of the ESCRT-III complex;furthermore,we established a new breast cancer survival prediction model based on cytoplasmic YAP1 expression.