直接注射法制作ICR小鼠肝癌原位移植瘤模型

目的：培养鼠肝癌H22细胞,直接注射法制作ICR小鼠肝癌原位移植瘤,为后续实验奠定基础。方法：鼠肝癌H22细胞体外培养,将调整好的对数生长期的肝癌细胞直接注射小鼠肝脏,2周后解剖观察,并进行组织HE染色。结果：所有实验小鼠均可见肿瘤生长,HE染色示肝细胞肝癌。结论：直接注射法制作ICR小鼠肝癌原位移植瘤模型简便易行,值得推广应用。     

直接注射法制作ICR 小鼠肝癌原位移植瘤模型

目的:培养鼠肝癌H22细胞,直接注射法制作ICR小鼠肝癌原位移植瘤,为后续实验奠定基础。方法:鼠肝癌H22细胞体外培养,将调整好的对数生长期的肝癌细胞直接注射小鼠肝脏,2周后解剖观察,并进行组织HE染色。结果:所有实验小鼠均可见肿瘤生长,HE染色示肝细胞肝癌。结论:直接注射法制作ICR小鼠肝癌原位移植瘤模型简便易行,值得推广应用。     

建立分泌型荧光素酶基因标记的原位肝癌模型及用于干扰素β基因治疗评价

旨在建立一种分泌型荧光素酶基因标记的小鼠原位移植型肝癌模型并观察其对干扰素β基因治疗的反应。首先建立稳定表达分泌型荧光素酶Gluc(Gaussia princeps luciferase)的小鼠肝癌细胞Hepa 1-6/Gluc;将该细胞通过脾注射至C57BL/6小鼠肝脏建立原位移植型肝癌模型,通过检测外周血Gluc活性监测小鼠体内肿瘤生长情况;用此模型观察水动力注射干扰素β质粒DNA的抗肿瘤效果。结果表明,通过脾注射Gluc基因标记的Hepa 1-6细胞可以建立小鼠原位移植型肝癌模型;外周血Gluc活性可以有效反映体内接种肿瘤细胞的数量和肿瘤的生长情况;通过监测外周血Gluc活性可灵敏反映干扰素β基因治疗对肿瘤生长的抑制作用。本研究表明,利用Gluc为报告基因建立的小鼠原位移植型肝癌模型可以体外实时监测肿瘤的生长情况,并能灵敏可靠地用于抗肿瘤治疗效果的评价。     

近交系小鼠移植性肝癌模型建立及对比分析

目的：通过对比分析选择建立原位移植性肝癌模型的最佳小鼠品系。方法选取C57、C3H和BALB／c各10只小鼠分别作为模型组Ⅰ、模型组Ⅱ和模型组Ⅲ,沿腹中线开腹后将H22细胞接种到各模型组小鼠肝脏实质内。于注射后第15天剖腹探查,观察各组成瘤率,测量腹水量和肿瘤体积,并进行肿瘤病理学分析。结果三组小鼠存活率均为100％,15天后三组小鼠均产生腹水,但三组腹水量之间不具有统计学差异。模型组Ⅰ小鼠肝癌移植成功率为100％,高于模型组Ⅱ的60％和模型组Ⅲ的30％。模型组Ⅰ小鼠肝脏肿瘤全部为大块紧实灰白色病灶,其肿瘤平均体积显著大于模型组Ⅱ和模型组Ⅲ（ P＜0.05）。病理结果证实三组小鼠肝脏的灰白色病灶均为原位肝细胞癌。结论 C57小鼠是复制原位移植性肝癌模型较为理想的实验动物,为今后研究原位肝癌的发病机制提供良好的实验平台。     

人肝癌裸小鼠常位移植实验研究

采用硫贲妥钠（３０ｍｇ／ｋｇ、３０％乙醇配制）麻醉和蘸上立止血（２５０ｋＩＵ／ｍｌ）的明胶海棉止血措施确保了人肝癌裸小鼠常位移植术能安全、可靠地进行。本中心建立的两株人肝癌裸小鼠移植瘤株（ＨＨＣ４、ＨＨＣ１５）已成功地移植于裸小鼠（ＳＰＦ级）肝脏内,移植瘤生长良好、传代稳定和持续分泌ＡＦＰ。荷瘤（ＨＨＣ１５）３～６周裸小鼠血清ＡＦＰ含量与瘤体积的增加呈正相关。常位移植前（７ｄ）裸小鼠皮下注射０．１ｍｌ０．５％ＣＣ１（Ｖ／Ｖ。橄榄油配制）能明显提高ＨＨＣ４常位移植的成功率（Ｘ２检验、Ｐ＜０．０１）;在微量ＣＣｌ４作用下,裸小鼠肝细胞受损伤,发生肝硬化,在此基础上所移植和生长的人肝癌常位移植瘤与大多数人肝癌病变发生的肝脏病理生理学特点相似,本模型的建立更适用于抗肝癌药物的模拟治疗和筛选。     

插线法制作大鼠局灶性脑缺血再灌流模型方法的改进

目的 探索插线法制作大鼠局灶性脑缺血再灌流模型方法的改进。方法 在前人制作模型方法基础上进行部分改进,用提线法阻断血流和在颈外动脉上剪小口进行插线。结果 缩短了手术时间,简化了模型制作过程,提高模型成功率。结论 本法复制插线法制作大鼠局灶性脑缺血再灌流模型,省时,操作简便,提高成功率。     

人鼠肝组织嵌合体模型的制备

目的研究制备人鼠肝组织嵌合小鼠模型。方法将人骨髓干细胞直接注射到一定日龄胎鼠肝组织,每只注射移植约1×109人骨髓干细胞。用免疫组化对出生一定日龄移植小鼠肝脏进行甲胎蛋白免疫组织化学检测,检定分析人肝细胞在小鼠体内嵌合生长情况。结果移植人骨髓干细胞胎鼠出生2月龄、12月龄可检测到甲胎蛋白。结论将人骨髓干细胞移植小鼠肝脏内能够存活并分化成人肝细胞并能够长期存活。     

基于临床肿瘤标本的胃癌转移模型建立

目的建立基于临床肿瘤标本的胃癌转移模型,为胃癌的转移研究提供个体化动物模型。方法将胃癌新鲜的手术标本移植到裸鼠皮下,建立胃癌患者异种移植(patient-derived xenograft,PDX)模型。进一步通过手术将皮下瘤组织原位移植到裸鼠胃部肌层,连续观察裸鼠的体征状态,通过近红外荧光活体成像技术检测肿瘤转移的发生。解剖荷瘤小鼠,将肺部转移灶进一步移植裸鼠皮下获得实体瘤。HE染色观察原发瘤与转移瘤的结构特征,(short tandem repeat) STR分析原发瘤和转移瘤的遗传特性。PCR-Array分析转移瘤和原发瘤中转移相关基因的表达。结果成功建立胃癌PDX模型,移植瘤组织结构与患者保持基本一致;通过胃部原位移植发现编号C19751的小鼠发生肺和肝的转移。其中肺转移灶皮下移植后获得了实体瘤,STR分析显示原发瘤保持了与肺转移瘤一致的遗传特征。PCR-Array结果显示,与原发瘤相比,转移瘤中CXCL12,IGF1和MMP2基因表达均显著上调。结论利用临床肿瘤标本成功建立胃癌转移模型,为胃癌转移研究提供了良好的个体化模型。     

小鼠腹部心脏移植模型的制作与改进

目的建立并改进小鼠腹部异位心脏移植模型,为器官移植研究提供技术支持。方法SPF级近交系小鼠112只进行心脏移植手术,在传统方法的基础上进行改进,观察改进后手术效果并分析其优势。结果手术成功率为89.28％。总手术时间（103.9±16.5）min,受体手术时间（73.0±7.9）min。改进的方法简化了操作步骤,降低了手术难度。结论改进的小鼠腹部异位心脏移植技术是一种简便、有效、成功率高的模型制作方法。     

转基因小鼠源性胰腺癌原位移植瘤模型的构建与评价

目的 构建转基因LSL-Kras^G12D/+LSL-Trp53^R172H/+Pdx1-Cre(KPC)小鼠胰腺癌原位移植瘤模型,为研究胰腺癌的发展机制和治疗策略提供稳定、可靠的药物临床前研究动物模型。方法 将KPC转基因小鼠的自发胰腺癌的组织块进行C57BL/6J小鼠胰腺原位移植,利用超声进行肿瘤监测,对原发肿瘤和传代肿瘤进行苏木精-伊红(HE)染色和免疫荧光染色评价模型的肿瘤病理学特征。结果 KPC小鼠的自发肿瘤能够在C57BL/6J小鼠的胰腺上稳定生长,肿瘤增殖指标Ki67、基质纤维化标志物α-SMA、免疫细胞标志物CD45和CD206均稳定表达,该模型能够稳定地保留原发胰腺癌病理学特征,并发生与临床胰腺癌患者相似的广泛转移。结论 成功建立转基因小鼠源性胰腺癌原位移植瘤模型,该模型能够模拟出胰腺癌的基质环境和免疫细胞浸润情况,具有较好的稳定性和均一性,可以作为研究胰腺癌进展和治疗策略的有效药物临床前研究模型。     

Wistar大鼠胶原诱导的关节炎造模因素的分析

目的通过比较不同的造模方法,分析影响胶原诱导关节炎（collagen-induced arthritis,CIA）大鼠模型建立的因素。方法选用Wistar大鼠造模,通过改变性别、剂量、年龄、注射部位及免疫方式,来比较造模成功率。结果不同性别、剂量、年龄及免疫方式造模成功率不同。结论4～5周龄Wistar雌性大鼠,初次免疫注射乳剂4点共0.20 mL,加强免疫在14 d之后3点共0.15 mL的造模成功率最高。     

miR-596-3p suppresses brain metastasis of non-small cell lung cancer by modulating YAP1 and IL-8

Brain metastasis (BM) frequently occurs in advanced non-small cell lung cancer (NSCLC) and is associated with poor clinical prognosis. Due to the location of metastatic lesions, the surgical resection is limited and the chemotherapy is ineffective because of the existence of the blood brain barrier (BBB). Therefore, it is essential to enhance our understanding about the underlying mechanisms associated with brain metastasis in NSCLC. In the present study, we explored the RNA-Seq data of brain metastasis cells from the GEO database, and extracted RNA collected from primary NSCLC tumors as well as paired brain metastatic lesions followed by microRNA PCR array. Meanwhile, we improved the in vivo model and constructed a cancer stem cell-derived transplantation model of brain metastasis in mice. Our data indicated that the level of miR-596-3p is high in primary NSCLC tumors, but significantly downregulated in the brain metastatic lesion. The prediction target of microRNA suggested that miR-596-3p was considered to modulate two genes essential in the brain invasion process, YAP1 and IL-8 that restrain the invasion of cancer cells and permeability of BBB, respectively. Moreover, in vivo experiments suggested that our model mimics the clinical aspect of NSCLC and improves the success ratio of brain metastasis model. The results demonstrated that miR-596-3p significantly inhibited the capacity of NSCLC cells to metastasize to the brain. Furthermore, these finding elucidated that miR-596-3p exerts a critical role in brain metastasis of NSCLC by modulating the YAP1-IL8 network, and this miRNA axis may provide a potential therapeutic strategy for brain metastasis.Subject terms: CNS cancer, miRNAs     

An improved intrafemoral injection with minimized leakage as an orthotopic mouse model of osteosarcoma

Osteosarcoma, the most common type of primary bone cancer, is the second highest cause of cancer-related death in pediatric patients. To understand the mechanisms behind osteosarcoma progression and to discover novel therapeutic strategies for this disease, a reliable and appropriate mouse model is essential. For this purpose, osteosarcoma cells need to be injected into the bone marrow. Previously, the intratibial and intrafemoral injection methods were reported; however, the major drawback of these methods is the potential leakage of tumor cells from the injection site during or after these procedures. To overcome this, we have established an improved method to minimize leakage in an orthotopic mouse model of osteosarcoma. By taking advantage of the anatomical benefits of the femur with less bowing and larger medullary cavity than those of the tibia, osteosarcoma cells are injected directly into the femoral cavity following reaming of its intramedullary space. To prevent potential leakage of tumor cells during and after the surgery, the injection site is sealed with bone wax. This method requires a minor surgery of approximately 15 min under anesthesia. Our established orthotopic osteosarcoma model could serve as a valuable and reliable tool for examining progression of various types of bone tumors.     

Impact of Tumor Localization and Method of Preoperative Biopsy on Sentinel Lymph Node Mapping After Periareolar Nuclide Injection

Background

To evaluate whether tumor localization and method of preoperative biopsy affect sentinel lymph node (SLN) detection after periareolar nuclide injection in breast cancer patients.

Methods and Findings

767 breast cancer patients were retrospectively included. For lymphscintigraphy periareolar nuclide injection was performed and the SLN was located by gamma camera. Patient and tumor characteristics were correlated to the success rate of SLN mapping. SLN marking failed in 9/61 (14.7%) patients with prior vacuum-assisted biopsy and 80/706 (11.3%) patients with prior core needle biopsy. Individually evaluated, biopsy method (p = 0.4) and tumor localization (p = 0.9) did not significantly affect the SLN detection rate. Patients with a vacuum-assisted biopsy of a tumor in the upper outer quadrant had a higher odds ratio of failing in SLN mapping (OR 3.8, p = 0.09) compared to core needle biopsy in the same localization (OR 0.9, p = 0.5).

Conclusions

Tumor localization and preoperative biopsy method do not significantly impact SLN mapping with periareolar nuclide injection. However, the failure risk tends to rise if vacuum-assisted biopsy of a tumor in the upper outer quadrant is performed.     

Quasi-likelihood estimation for relative risk regression models

For a prospective randomized clinical trial with two groups, the relative risk can be used as a measure of treatment effect and is directly interpretable as the ratio of success probabilities in the new treatment group versus the placebo group. For a prospective study with many covariates and a binary outcome (success or failure), relative risk regression may be of interest. If we model the log of the success probability as a linear function of covariates, the regression coefficients are log-relative risks. However, using such a log-linear model with a Bernoulli likelihood can lead to convergence problems in the Newton-Raphson algorithm. This is likely to occur when the success probabilities are close to one. A constrained likelihood method proposed by Wacholder (1986, American Journal of Epidemiology 123, 174-184), also has convergence problems. We propose a quasi-likelihood method of moments technique in which we naively assume the Bernoulli outcome is Poisson, with the mean (success probability) following a log-linear model. We use the Poisson maximum likelihood equations to estimate the regression coefficients without constraints. Using method of moment ideas, one can show that the estimates using the Poisson likelihood will be consistent and asymptotically normal. We apply these methods to a double-blinded randomized trial in primary biliary cirrhosis of the liver (Markus et al., 1989, New England Journal of Medicine 320, 1709-1713).     

糖尿病高血压大鼠动物模型的制备及稳定性观察

目的：探讨建立高血压合并糖尿病（DiabetesMellitus,DM）大鼠模型的方法,并观察模型的稳定性。方法：采用链脲佐菌素（Streptozotocin,STZ）腹腔注射的方法造模。8周龄的SHR大鼠（spontaneouslyhypertensiverats）16只,随机等分成对照组和造模组。另选8只8周龄WKY大鼠作为正常血压对照组。给予造模组SHR按55mg/kg体重的剂量腹腔注射STZ,诱导建立糖尿病高血压大鼠动物模型。结果：小剂量STZ（55mg/kg）腹腔注射SHR制备的糖尿病高血压大鼠模型,造模成本低,成模率高,模型稳定。结论：造模组能成功诱导建立糖尿病高血压大鼠模型。     

Microinjection of living adherent cells by using a semi-automatic microinjection system

Testing in vitro is an alternative to animal experimentation. The capillary pressure microinjection technique is a supporting technology for efficient in vitro testing. The main benefit of the technique is the possibility of injecting large molecules into a single living cell. The ultimate goal of the research discussed in this paper is to increase the cell survival rate in capillary pressure microinjection. A method to reliably evaluate cell survival rate is therefore needed. A three-phase evaluation process is presented in this paper. The first phase determines the success rate of the injection capillary to penetrate the cell membrane. The second phase studies the success rate of delivering the injection substance inside the cell, while the third phase studies cell survival after the microinjection. In addition to the three-phase evaluation process, this paper describes the initial results of penetration and injection tests performed by using a semi-automatic capillary pressure microinjection system developed by the research group. Three adherent cell lines, namely, retinal pigment epithelial cells, MCF-7 human breast cancer cells and SH-SY5Y neuroblastoma cells, were used in the experiments. The results of the penetration tests show that the average success rate of penetrating the cell membrane using the micromanipulator was 87%. The goal of the injection tests was to demonstrate the successful microinjection of living cells and to study the injection success rate. Fluorescein dextran was injected into MCF-7 cells, and preliminary results showed an injection success rate of 49%. In the survival tests, the neuronal cells were microinjected with KCl. During long-term observation after the microinjection, the microinjected cells first decreased their adhesion to the plate, but later adhered to the bottom of the plate and even grew some dendrites. In the next phase of the study, more tests will be performed in order to obtain a statistically reliable value for the survival rate.     

Therapeutic efficacy of melanoma-reactive TIL injected in stage III melanoma patients

Adoptive therapy for cancer using tumor-infiltrating lymphocytes (TIL) has mainly been investigated in cancer patients with advanced stage disease. The limited clinical success has not been encouraging, although this might be explained by poor TIL specificity and/or high tumor burden. To re-evaluate the effectiveness of adoptive therapy, we analyzed the capacity of tumor-reactive TIL injection in preventing the further development of disease in stage III melanoma patients after complete tumor resection. A phase II/III randomized trial was performed on 88 melanoma patients, who received autologous TIL plus interleukin-2 (IL-2) or IL-2 only. The duration of relapse-free survival was analyzed, taking into account the immunological specificity of injected TIL and the number of metastatic lymph nodes removed before treatment. Kaplan-Meyer analysis revealed that the injection of tumor-reactive TIL was statistically correlated with prolonged relapse-free survival in patients with only one metastatic lymph node. Therefore, improved clinical outcome could be obtained after adoptive therapy by selecting appropriate groups of patients and monitoring the specificity of the injected TIL populations.     

Development of an orthotopic human pancreatic cancer xenograft model using ultrasound guided injection of cells

Mice have been employed as models of cancer for over a century, providing significant advances in our understanding of this multifaceted family of diseases. In particular, orthotopic tumor xenograft mouse models are emerging as the preference for cancer research due to increased clinical relevance over subcutaneous mouse models. In the current study, we developed orthotopic pancreatic cancer xenograft models in mice by a minimally invasive method, ultrasound guided injection (USGI) comparable to highly invasive surgical orthotopic injection (SOI) methods. This optimized method prevented injection complications such as recoil of cells through the injection canal or leakage of cells out of the pancreas into the peritoneal cavity. Tumor growth was monitored in vivo and quantified by ultrasound imaging weekly, tumors were also detected by in vivo fluorescence imaging using a tumor targeted molecular probe. The mean tumor volumes for the USGI and SOI models after 2 weeks of tumor growth were 205 mm(3) and 178 mm(3) respectively. By USGI of human pancreatic cancer cell lines, human orthotopic pancreatic cancer xenografts were established. Based on ultrasound imaging, the orthotopic human pancreatic cancer xenograft take rate was 100% for both human pancreatic cancer cell lines used, MiaPaCa-2 and Su86.86, with mean tumor volumes of 28 mm(3)and 30 mm(3). We demonstrated that this USGI method is feasible, reproducible, facile, minimally invasive and improved compared to the highly-invasive SOI method for establishing orthotopic pancreatic tumor xenograft models suitable for molecular imaging.     

用改进的细胞核移植方法构建重构胚

为了能够找出一种既容易操作,又不需要特殊设备的核移植方法,对以前的操作进行了改进。首先以预先吸有细胞核或细胞的注射针在固定于持卵针上的卵母细胞透明带上穿刺两个孔,然后一边缓慢地将注射针回拔至卵周隙中,一边逐渐增加持卵针中的负压,直至极体与目标核质被完整吸入持卵针中而完成去核,最后在不拔出注射针的情况下直接注射细胞核或完整细胞进而完成重构胚的构建。用此方法对200个卵母细胞进行注核和注细胞操作,平均完成一个重构胚的构建各自耗时约40s和30s,成功率分别为62.6%和86.0%。用核染料Hoechst 33342 对卵母细胞的去核效率进行验证,去核成功率达到73.3%。实验证明,用此方法可以在只有倒置显微镜和显微操作仪的条件下一次性快速完成去核和注核,大大提高了细胞核移植的效率和重构胚成活率;更重要的是该方法操作简单,新手可以很快掌握该技术,易于在实际工作中推广应用。