无菌动物及其有关实验动物知识

无菌动物(germfree animal)是一种新型的实验动物。普通的实验动物都受到自然界微生物或寄生虫的侵袭,有的外观健康其实却隐藏着某种疾病。用普通动物做实验,敏感性差,实验结果缺乏再现性。要提高动物实验的准确性就要对实验动物在遗传和微生物两个方面加以控制,努力提高其均一性。由兄妹间近亲交配繁殖20代以上建立的纯品系动物,个体差异小,实验结果比较准确。但是,用纯品系动物做实验还没有排除自然感染的微生物和寄生虫的     

小鼠主要脑区组织的优化急性分离法

实验小鼠具有体型小,基因特性明确,转基因或突变体品系多,饲养方便,繁殖迅速等优点,已被广泛应用于现代生物学、医学、药理学和心理学研究。在大量采用小鼠为受试对象的同时,国内外研究者也越来越重视实验动物的保护。最大限度地利用实验动物,并尽可能地减少动物使用量,这也是国内外实验室一直追求并建立的理念。本文总结了本实验室快速分离获取小鼠不同脑区新鲜组织用于蛋白免疫印迹和神经细胞培养的经验,旨在为实验初学者提供指导的同时,也为提高实验动物的利用率和降低动物使用数量提供思路和方法。     

美国实验动物品种资源现状分析

实验动物是生命科学和生物医药创新研究等重要的支撑条件。随着生命科学和生物医药产业的快速发展,实验动物、动物模型资源数量和种类都快速增加。据统计,世界各地共培育着200多种共计26 000多个品系的实验动物,其中有2607个品系为常规实验动物。美国是世界上实验动物资源大国,拥有最全的实验动物品系品种资源和保藏机构。本文首次对美国实验动物资源进行了系统分析归类,以便为我国实验动物资源发展提供借鉴。     

小鼠生长曲线与应用

在实验动物的繁殖中,我们发现同品系同龄的动物体重差异较大;在动物实验中也观察到动物的个体差异性。为此,我们就不同性别动物的体重与年龄的关系进行了实验观察。1 方法和结果选用引自中国医学科学院实验动物中心、已在我中心SPF屏障系统繁育10代之SPF级近交系CBA/J/Ola小鼠,以21日龄离乳鼠16窝48只,分雌(21只)雄(27只)两     

国家啮齿类实验动物种子中心

国家啮齿类实验动物种子中心是 1998年由国家科委批准建立的 ,设在中国药品生物制品检定所实验动物中心。其主要任务是 :引进、收集和保存实验动物品种、品系 ;研究实验动物保种新技术 ;培育实验动物新品种、品系 ;为国内外用户提供标准的实验动物种子。我中心建立以来 ,已经向全国二十个省市的 5 0多家单位 ,供应了SPF级种鼠一万多只。目前保存有SPF级大小鼠、豚鼠、家兔等 2 0多个品种品系的实验动物 ,最近引入了F344、B N、ICR、C57BL 10等品系 ,还将陆续从国外引进急需的实验动物种子。我中心严格控制实验动物质量 ,确保为用户提…     

国家啮齿类实验动物种子中心简介

国家啮齿类实验动物种子中心是1 998年由国家科委批准建立的,设在中国药品生物制品检定所实验动物中心。其主要任务是:引进、收集和保存实验动物品种、品系;研究实验动物保种新技术;培育实验动物新品种、品系;为国内外用户提供标准的实验动物种子。该中心建立以来,已经向全国2 0个省市的5 0多家单位,供应了SPF级种鼠1万多只。目前保存有SPF级大、小鼠,豚鼠,家兔等2 0多个品种品系的实验动物,最近引入了F344、B .N、ICR、C57BL 1 0等品系,还将陆续从国外引进急需的实验动物种子。该中心严格控制实验动物质量,确保为用户提供合格的种子;…     

疟疾媒介斯氏按蚊印度品系经溴氰菊酯或溴氰菊酯增效剂选择后的繁殖劣势

了解敏感和抗性蚊虫的繁殖适合度对于规划和实施蚊虫防治计划具有重要意义。本研究分别将斯氏按蚊Anopheles stephensi幼虫用溴氰菊酯(AnD_L)及溴氰菊酯和PBO混配制剂(1∶5) (AnD_P), 或斯氏按蚊成虫用溴氰菊酯(AnD_A) 进行选择后, 在实验室内检测了起源于印度德里的斯氏按蚊亲本（AnS）和抗性品系 (AnR) 的繁殖适合度的变化,从繁殖力、生育力、卵孵化率和生殖营养周期的长度等方面评价了斯氏按蚊的繁殖适合度。结果表明：与AnS品系相比, AnR品系的生殖营养周期缩短了60%~73%。与AnS品系相比, AnR品系的产卵量显著降低, 降幅达14.5%~37.9%,对溴氰菊酯抗性最强的AnD_L40品系的产卵量降低得最多。这些结果说明溴氰菊酯抗性与繁殖劣势之间可能存在正相关。与亲本品系相比, AnD_L40品系的卵孵化率降低了19.4%~30.9%, 进一步证实了这一相关性。在RD_P品系中观察到繁殖适合度降低, 表明溴氰菊酯增效剂的选择不仅在降低溴氰菊酯抗性水平而且在降低抗性个体频率上的效率。在对溴氰菊酯几乎不具有抗性的成虫品系的选择中繁殖适合度降低, 暗示溴氰菊酯作为灭杀斯氏按蚊成虫剂的效果要好于作为杀幼虫剂的效果。这些结果提示, 通过对斯氏按蚊实施不同抗性治理策略, 种群中抗性基因型的繁殖适合度的降低可消除杂合子和抗性纯合子。     

PCR扩增近交系大鼠微卫星位点DNA多态性的研究

本实验选取大鼠7条染色体上的微卫星位点合成了10对引物,利用聚合酶链反应（PCR）扩增技术对国内北京和哈尔滨等4家单位提供伯6个品系（SHR、SHRSP、LEW、RCS、WKY和F344）的8个近交系大鼠群体进行了DNA多态性分析的研究。结果表明：9个微卫星位点具有显多态性;不同品系个体之间具有多态性;同一群体不同个体之间除SHR（哈）的SMST位点和WKY（哈）的AGT位点出现一定的差异,其他均没有差异;不同地区同一品系的不同个体之间也存在一定的差异。该方法能有效地对近交系与杂交系、品系与品系、品系与亚系加以区分。因此,本实验为开展近交系大鼠遗传作图、基因定位和为实验动物的遗传背景监测提供可靠的信息,为大鼠遗传基因的研究提供了一个快速简例、特异准确的方法。     

棉铃虫对氰戊菊酯抗性品系和敏感品系的相对适合度

通过构建棉铃虫Helicoverpa armigera(Hubner)对氰戊菊酯抗性品系(Fen-R)和敏感品系(S)的实验种群生命表,比较了一系列生长发育和繁殖特征,并用净增殖率(Rn)来确定两个品系的相对适合度。 结果表明,Fen-R品系与敏感品系相比具有一定程度的繁殖不利性,包括雌蛾交配率降低,每头雌蛾的平均产卵量减少以及较低的卵孵化率;没有观察到Fen-R品系在生长发育上的不利性。Fen-R品系相对于敏感品系具有0.69的适合度。     

小家鼠和实验小鼠遗传特性的比较研究

本文用同工酶电泳法、微量细胞毒法和免疫双向扩散法对我国4个动物地理区的6个采集点的156个小家鼠(Mus musculus)进行了遗传特性的调查。结果发现:在全部被测的13个位点中,小家鼠在7个位点上存在着多种实验小鼠中罕见的基因组成;而不同动物地理区和亚区的小家鼠的遗传特性又各不相同。从而指出将小家鼠的特有基因导入实验小鼠,培育新品系的重大意义。     

A computer program that draws pedigree charts for inbred strains of animals

We produced a computer program that draws pedigree charts for inbred strains of animals such as mice or rats. This program is composed of four subprograms, which are (1) inputting the data, (2) drawing pedigree charts, (3) listing the data which have been input, and (4) backup of the system and the data. Pedigree charts and lists of data can be displayed on a TV screen and printed out on the papers. Using this program, we drew the pedigree charts of the inbred strains of rats which we are maintaining by brother-sister inbreeding in our institute and found that there were three sublines in one of the strains, WKAH/Hkm, because of unsuitable maintenance. This program is very convenient to draw the pedigree charts and useful for checking the maintenance of inbred strains or the strains of animal models of human diseases.     

Variation in pentobarbitone sleeping time in mice. 2. Variables affecting test results

The effect of some environmental factors on the pentobarbitone sleeping time (PST) in inbred strains of mice has been investigated. Age, dose level and fasting before the test significantly altered the PST while the source of the drug and regular handling of the mice had no effect. None of these factors affected strains differentially. Unsystematic effects such as litter differences contributed only a small proportion of the total variation in the experiments. The strain rankings were different from those obtained in some previous experiments. The effects of some of the environmental factors on the PST did not always agree with previous work. The implications of these results for the design of similar experiments and the relevance of baseline values in laboratory animals are discussed.     

Microbiological monitoring in inbred mouse foundation stocks in Japan

Microbiological monitoring on 128 inbred mouse foundation stocks consisted of common 10 inbred strains and inbred strains originated from outbred dd mice was performed by cooperation of 24 organizations. A total of 881 mice were divided into 647 conventional animals from 95 colonies and 234 barrier-sustained animals from 33 colonies. Three viral, one mycoplasmal, 6 bacterial, one fungal and 3 parasitic agents selected as monitoring microbes according to the proposed selection standards. Among conventional colonies, 84.2% were positive for at least one agent. The highest detection rate was 44.2% for S. obvelata, followed by P. pneumotropica and S. muris, P. aeruginosa, G. muris, Sendai virus, M. pulmonis, MHV and E. coli O115a, c: K (B). Of these agents, only one microbe, P. aeruginosa, was detected in barrier-sustained colonies (36.4%), thus the efficacy of barrier system for the microbiological quality control of the inbred mouse foundation stocks was actually demonstrated. The positive rates of MHV (6.3%) and Sendai v. (16.8%) were significantly low compared with those in experimental mouse colonies. Positivity for parasites was rather high and they were infested together with other pathogens in many cases. Thus parasites including G. muris, S. muris and S. obvelata were regarded as useful indicators to see microbiological contaminations in conventional mice. There observed no strain difference in susceptibility to pathogens except for C57BL/6 and AKR mice which seemed to be high antibody responders to MHV.     

A third component causing random variability beside environment and genotype. A reason for the limited success of a 30 year long effort to standardize laboratory animals?

This paper is a review of experiments, performed in our laboratory during the past 20 years, designed to analyse the significance of different components of random variability in quantitative traits in laboratory rats and mice. Reduction of genetic variability by using inbred strains and reduction of environmental variability by highly standardized husbandry in laboratory animals did not remarkably reduce the range of random variability in quantitative biological traits. Neither did a tremendous increase of the environmental variability (i.e., living in a natural setting) increase it. Therefore, the postnatal environment cannot be that important as the source of random variability. Utilizing methods established in twin research, only 20-30% of the range of the body weight in inbred mice were directly estimated to be of environmental origin. The remaining 70-80% were due to a third component creating biological random variability, in addition to the genetic and environmental influences. This third component is effective at or before fertilization and may originate from ooplasmic differences. It is the most important component of the phenotypic random variability, fixing its range and dominating the genetic and the environmental component. The Gaussian distribution of the body weights observed, even in inbred animals, seems to be an arrangement supporting natural selection rather than the consequence of heterogeneous environmental influences. In a group of inbred rats, the males with the highest chance of parenting the next generation were gathered in the central classes of the distribution of the body weight.     

A locus that enhances the induction of endogenous ecotropic murine leukemia viruses is distinct from genome-length ecotropic proviruses.

The segregation of genes that enhance the induction of ecotropic murine leukemia viruses (In loci) has been compared with the segregation of ecotropic-specific nucleotide sequences in 12 low-leukemic mouse strains and 18 recombinant inbred strains. Endogenous ecotropic viruses of these strains are of genome length and structurally similar to AKR ecotropic proviruses. Low-leukemic strains of related pedigree contain ecotropic proviruses at common integration sites. Loci previously identified which enhance induction of ecotropic viruses (In genes) were correlated with the inheritance of ecotropic viral sequences in inbred low-leukemic mouse strains and in CXB recombinant inbred mouse strains. However, four BXH recombinant inbred strains were observed to possess an In gene(s) yet lack the probed envelope gene region for the corresponding endogenous ecotropic virus. These observations indicate that at least one gene that enhances ecotropic virus expression in vitro is encoded by DNA sequences outside ecotropic proviruses or by subgenomic viral sequences.     

Genotype-specific environmental impact on the variance of blood values in inbred and F1 hybrid mice

Mice are important models for biomedical research because of the possibility of standardizing genetic background and environmental conditions, which both affect phenotypic variability. Inbred mouse strains as well as F₁ hybrid mice are routinely used as genetically defined animal models; however, only a few studies investigated the variance of phenotypic parameters in inbred versus F₁ hybrid mice and the potential interference of the genetic background with different housing conditions. Thus, we analyzed the ranges of clinical chemical and hematologic parameters in C3H and C57BL/6 inbred mice and their reciprocal F₁ hybrids (B6C3F1, C3B6F1) in two different mouse facilities. Two thirds of the blood parameters examined in the same strain differed between the facilities for both the inbred strains and the F₁ hybrid lines. The relation of the values between inbred and F₁ hybrid mice was also affected by the facility. The variance of blood parameters in F₁ hybrid mice compared with their parental inbred strains was inconsistent in one facility but generally smaller in the other facility. A subsequent study of F₁ hybrid animals derived from the parental strains C3H and BALB/c, which was done in the latter housing unit, detected no general difference in the variance of blood parameters between F₁ hybrid and inbred mice. Our study clearly demonstrates the possibility of major interactions between genotype and environment regarding the variance of clinical chemical and hematologic parameters.     

Female expression of the H-2-linked sex-limited protein (Slp) due to non-H-2 genes

Female mice of 15 inbred strains in which males express the H-2-linked sex-limited protein (Slp) were tested for the production of this protein. Four inbred strains (FM, LG/J, NZB, PL/J) were found in which females produce Slp in the absence of hormonal manipulation. Crosses have been made between strains FM, NZB, or PL/J and several Slp-negative strains. Slp-typing of the F₁, F₂, and backcross progeny, as well as of a number of recombinant inbred strains, indicates that production of Slp by normal females of these strains depends upon the concurrent presence of an Slp-positive,H-t2-linked allele and of permissive alleles of one or two non-H-2 autosomal genes. Complementation studies with two of the strains (FM and PL) indicate that an identical genetic mechanism mediates expression of Slp in females of these two strains. FM-derived animals carrying the testicular feminization mutation (tfm) also express Slp, as do castrated NZB mice, indicating that Slp expression in these instances is not dependent upon testosterone as it is in other inbred strains. It is concluded from these results that genes distinct from the putative structural gene for Slp influence the sex-limitation of its expression.     

SNP genotyping for the genetic monitoring of laboratory mice by using a microarray-based method with dualcolour fluorescence hybridisation

Ensuring the genetic homogeneity of the mice used in laboratory experiments contributes to the Reduction aspect of the Three Rs, by maximising the quality of the data obtained from any animals that are used for these purposes, and ultimately reducing the numbers of animals used. Single nucleotide polymorphism (SNP) genotyping is especially suitable for use in the analysis of the genetic purity of model organisms such as the mouse, because bi-allelic markers remain fully informative when used to characterise crosses between inbred strains. Here, we attempted to apply a microarray-based method for a SNP marker to monitor the genetic quality of inbred mouse strains, so as to validate the reliability, stability and applicability of this SNP genotyping panel. The amplified PCR products containing four different SNP loci from four inbred mouse strains were spotted and immobilised onto amino-modified glass slides to generate a microarray. This was then interrogated through hybridisation with dual-colour probes, to determine the SNP genotypes of each sample. The results indicated that this microarray-based method could effectively determine the genotypes of the four selected SNPs with a high degree of accuracy. We have developed a new SNP genotyping technique for effective use in the genetic monitoring of inbred mouse strains.     

Inbred and outbred mice have equivalent variability in a cockroach allergen-induced model of asthma

Outbred mice traditionally are considered to display high variability, thereby limiting their use in some studies. Researchers frequently are encouraged to use inbred strains of mice because of the greater homogeneity of these experimental animals. We compared the pulmonary inflammatory response of inbred BALB/cJ mice to that of outbred HSD-ICR mice by measuring multiple variables, including cytokines, chemokines, number of pulmonary inflammatory cells, and respiratory parameters. Cockroach allergens induced significant pulmonary inflammation in both BALB and ICR mice. Our comparisons of the coefficients of variance for 148 discrete data sets for each strain or stock indicated that BALB and ICR mice have roughly equivalent intrastrain or -stock variability in our model of asthma-like pulmonary inflammation. The average coefficient of variance, calculated as the ratio of the SD to the mean of a data set, was 0.35 ± 0.34 for BALB mice compared with 0.31 ± 0.32 for ICR mice. In conclusion, inbred BALB and outbred ICR mice have roughly equivalent intrastrain or -stock variability in a murine model of asthma-like pulmonary inflammation.     

Physical performance and soleus muscle fiber composition in wild-derived and laboratory inbred mouse strains.

We compared four inbred mouse strains in their physical performance, measured as a maximal treadmill running time, characteristics of soleus muscle, anatomic character, and growth. The strains used were Mus musculus domesticus [C57BL/6 (B6) and BALB/c], Mus musculus molossinus (MSM/Ms), and Mus spretus. Maximal running time was significantly different among these four mouse strains. Running time until exhaustion was highest in MSM/Ms and lowest in M. spretus. Maximal times for the laboratory mouse strains were nearly identical. Soleus muscle fiber type and cross-sectional area also differed significantly among the species. In particular, M. spretus was significantly different from the other inbred mouse strains. Growth in the wild-derived inbred mice appeared to be complete earlier than in the laboratory mice, and the body size of the wild strains was about half that of the laboratory strains. From these results, we propose that wild-derived inbred mouse strains are useful models for enhancing phenotypic variation in physical performance and adaptability.