高压氧对正常及SIRS大鼠脾T淋巴细胞的影响

本实验以SIRS为基础,以免疫功能和炎症反应中具有代表性的脾T淋巴细胞为研究对象,观察高压氧对正常机体以及SIRS状态机体的影响并探讨其可能的机制。健康雄性SD大鼠40只,体重约140~180 g,随机分为5组,每组8只。A组：腹腔注射生理盐水（5 mL/kg）;B组：腹腔注射等量生理盐水,做3次高压氧;C组：腹腔注射酵母多糖-石蜡悬液（500 mg/kg）;D组：腹腔注射酵母多糖-石蜡悬液（500 mg/kg）,做1次高压氧治疗;E组：腹腔注射酵母多糖-石蜡悬液（500 mg/kg）,做3次高压氧治疗。采用流式细胞仪计算大鼠脾脏淋巴细胞数量及比例。高压氧治疗（B组）降低正常大鼠外周血CD4＋T细胞百分比（P〈0.01）,对CD8＋T细胞无影响,因此CD4＋/CD8＋T细胞比值下降（P〈0.05）。酵母多糖腹腔注射（C组）使大鼠外周血CD4＋、CD8＋T细胞均减少（P〈0.01）,但CD4＋/CD8＋T细胞比值不变。1次和3次HBO治疗（D和E组）可使酵母多糖所致CD4＋T细胞减少（C组）明显恢复（P〈0.01,P〈0.05）,故CD3＋CD4＋/CD3＋CD8＋比值升高（P〈0.01,P〈0.05）,HBO几乎不影响CD8＋T细胞比例（P〉0.05）。酵母多糖导致大鼠脾脏CD4＋和CD8＋T细胞比例减少;高压氧可减少正常大鼠脾脏CD4＋T细胞比例,而增加SIRS脾脏的CD4＋T细胞比例,而对CD8＋T细胞无影响。     

微卫星DNA标记在近交系大鼠HFJ和MIJ遗传监测中的应用

目的 用24对引物对近交系HFJ和MIJ大鼠的微卫星位点进行多态性分析,并选用近交系Lewis和F344大鼠作为对照,进行比较分析.方法 用传统的酚-氯仿法分别提取4个近交系大鼠MIJ、HFJ、Lewis和F344 的基因组DNA,选取大鼠24个微卫星位点,通过PCR扩增,扩增产物经过非变性聚丙烯酰胺凝胶电泳和银染,根据电泳结果,比较分析4种品系近交系大鼠之间微卫星多态性.结果 4种品系及品系内不同个体的近交系大鼠在24个微卫星位点上的扩增产物均出现一个条带,MIJ和HFJ大鼠在品系间和品系内均表现为单态性,同Lewis 和F344的扩增结果比较,14个位点显示多态性,有10个位点显示单态性.结论 两个近交系大鼠品系MIJ和HFJ符合近交系要求,筛选出的14个多态性微卫星位点可用于有关近交系大鼠的遗传背景监测.     

CD8＋CD122＋T细胞在脑缺血过程中作用的研究

目的：探讨CD8＋CD122＋T细胞在脑缺血过程中的作用及其机制。方法：线栓法建立小鼠大脑中动脉栓塞模型（MCAO）;激光共聚焦显微镜检测小鼠脑缺血组织中CD8＋CD122＋T细胞浸润情况;流式细胞仪检测脑缺血组织中CD8＋CD122＋T细胞／CD3＋T细胞的比例及脾和胸腺中CD8＋CD12TT细胞数量变化;RT—PCR方法检测CD8＋CD122＋T细胞对氧糖剥夺（Oxygen—glucosedeprivation,OGD）条件下星形胶质细胞表达TNF-α,IL-1β,IFN-γ的影响。结果：各时间点脑缺血组织中均有CD8＋CD122＋T胞浸润,且随脑缺血时间延长,缺血侧脑组织中CD8＋CD122＋T细胞／CD3＋T细胞比例逐渐增加,5d和7d组差异显著,与非缺血侧相比,P5d〈0．05,P7d〈0．05;MCAO小鼠脾及胸腺中CD8＋CD122＋T细胞呈现先增高后降低的趋势。星形胶质细胞经OGD处理后,与对照组相比,IFN-γ、TNF-α、IL—1β表达显著增高,PIFN-γ〈0．01、PTNF-α〈0．001、PIL-1β〈0．01;CD122-blocked组与CD8＋组相比,IFN-γ、TNF-α、IL-1β表达明显增高,PIFN-γ〈0．05、PINF-α〈0．05、PIL-1β〈0．01;CD8＋组与HBSS组相比,IFN-γ表达降低,P〈0．05;IL-1β表达有降低的趋势。结论：CD8＋CD122可细胞在脑缺血过程中发挥保护性作用,其保护作用通过CD122抑制星形胶质细胞TNF-α,IL-1β,IFN-γ炎症因子表达实现的。     

CD4＋CD25＋FoxP3＋调节性T细胞与黑龙江省HIV／AIDS患者病情相关性的研究

目的：比较黑龙江省H1V／AIDS患者与健康对照者（healthy controls,HCs）外周血cD4＋CD25＋F0xP3＋调节性T细胞数量、免疫抑制功能的变化,探讨CD4＋CD25＋FoxP3＋调节性T细胞在HIV／AIDS感染过程中的作用。方法：采用流式细胞仪检测21例HIV／AIDS患者及20例健康对照组的外周血CD4＋CD25＋FoxP3＋调节性T细胞数量的百分比及绝对数量;采用共同培养方法检测HIV／AIDS患者外周血cD4℃D25十FoxP3＋调节性T细胞免疫抑制功能的变化;实时荧光定量聚合酶链反应（RT-FQ-PCR）检测HIV／AIDS患者外周血CD4＋CD25＋FoxP3＋调节性T细胞中FoxP3mRNA的表达。结果：黑龙江省HIV／AIDS患者外周血CD4＋CD25下oxP3＋调节性T细胞比率明显高于HCs（P〈O．01）,而CD4-CD25＋FoxP3＋调节性T细胞的绝对计数显著下降,且与CD4＋T细胞绝对计数成反比;混合淋巴细胞共同培养结果显示,HIV／AIDS患者外周血CD4＋CD25＋FoxP3＋调节性T细胞的抑制功能无明显变化;HIV／AIDS患者外周血CD4＋CD25＋FoxP3＋调节性T细胞的FoxP3mRNA相对表达量无显著变化。结论：黑龙江省HIV／AIDS患者cD4℃D25＋FoxP3＋调节性T细胞的数量变化与病情相关。     

肿瘤患者CD8+T细胞中CD28表达的研究进展

CD28与B7结合形成的共刺激信号是T细胞激活的第二信号,肿瘤患者CD8^＋T细胞上CD28分子在肿瘤免疫中发挥着重要作用。人体抗肿瘤免疫主要由CD8^＋T细胞介导,根据CD28的表达与否可将CD8^＋T细胞分为细胞毒T细胞（CD8^＋CD28^＋,CTL）和抑制性T细胞（CD8^＋C28^-,Ts）。CTL是体内杀伤肿瘤细胞的主要功能性细胞之一,当该细胞与肿瘤接触时,通过共刺激信号而被激活,发挥其对肿瘤细胞的杀伤作用;Ts在机体的免疫耐受中发挥作用。现就肿瘤患者CD8^＋T细胞上CD28的表达作一综述。     

SIVmac239病毒经不同途径感染恒河猴急性期CD4~＋T细胞数量与其细胞表面CD95表达量的变化关系

目的研究SIVmac239病毒分别通过直肠（rectal infection：IR）及静脉（intravenous infection：IV）感染恒河猴,在感染急性期外周血CD4＋T细胞数量与其细胞表面的死亡受体（CD95）表达量之间的变化关系。方法将SIVmac239经直肠及静脉途径各感染14只恒河猴。监测病毒载量、CD4＋T淋巴细胞数量及CD4＋/CD8＋比值的变化,从而明确感染。同时,在感染急性期内9个时间点采集静脉血,并利用流式细胞术分析CD4＋T细胞表面CD95的表达量。结果静脉组恒河猴CD95表达量于第2天开始升高,第7天达到最高,同时CD4＋T淋巴细胞数降到最低。直肠组恒河猴也于感染后第2天开始升高,但第10天才达到最高值,CD4＋T淋巴细胞数于第17天降到最低。同静脉组相比,直肠组CD95表达量增高及CD4＋T细胞数降低均较晚出现,且其CD4＋T细胞数量降至最低晚于CD95表达量达到峰值一周后出现。结论 SIVmac239经直肠及静脉感染恒河猴后,伴随CD4＋T细胞表面CD95表达的升高,CD4＋T细胞数量逐渐下降。但不同感染途径对CD4＋T细胞表面CD95的表达量与CD4＋T淋巴细胞数的变化不尽相同,这可能由于不同感染途径造成CD95在感染急性期CD4＋T细胞数量降低中发挥的作用不同。     

外周血CD4^＋、CD8^＋及CD56^＋细胞在肺癌靶向治疗患者中的表达意义

目的：探讨埃罗替尼靶向治疗前后非小细胞肺癌患者外周血CD4^＋,CD8^＋和CD56^＋的表达及其临床意义。方法：流式技术检测30例EGFR突变的非小细胞肺癌患者埃罗替尼一线靶向治疗前后,外周血T细胞亚群的表达情况及疗效。结果：靶向治疗1个月后,与治疗前相比较非小细胞肺癌患者外周血T细胞亚群CD4^＋CD8^＋以及CD56^＋表达数量有统计学差异（P〈0．05）。其中,CD4^＋表达上升,CD8^＋和CD56^＋表达下降。结论：埃罗替尼靶向治疗可以改善非小细胞肺癌患者细胞免疫功能,观察外周血T细胞亚群表达情况有助于评价埃罗替尼靶向治疗的疗效和预后。     

CD40L启动CD4^＋T细胞缺乏小鼠免疫反应的研究

随着HIV感染者及各类医疗措施导致的免疫受损者的增多,探讨一种适合免疫缺陷人群的预防机会感染的策略越来越受到重视。研究表明,CD4^＋T细胞是抵抗肺孢子菌等机会感染的最主要因素,但不是唯一的因素。其中CD40配体（CD40L）被认为是一种可以启动B细胞和CD8^＋T细胞反应的关键因子。为探讨CD4^＋L是否能在缺乏CD4^＋T细胞的小鼠体内启动免疫反应,本文研究了用卵白蛋白（OVA）作为模型抗原,联合应用CD40L引起的免疫反应。结果显示,同时应用OVA和CD40L,可使CD4^＋T细胞耗竭小鼠体内抗OVA IgG抗体和抗原特异性IFN明显增多,提示在CD4^＋T细胞缺乏的宿主体内,CIMOL可以启动B细胞和CD8^＋T细胞类免疫反应。该结果为抗肺孢子菌等机会性感染的免疫预防研究提供可贵的资料。     

siRNA沉默t-bet基因对CD4、CD8T淋巴细胞亚群IFN-γ产生的影响

利用化学合成针对人t-bet基因的小干扰RNA（siRNA）,转染体外培养的人外周血单个核细胞,利用流式细胞仪分选纯化CD4^＋、CD8^＋T淋巴细胞,半定量RT-PCR检测CD4^＋、CD8^＋T淋巴细胞中t-betmRNA的表达变化,流式细胞术检测转染前后IFN-γ产生的变化情况。探讨转录因子t-bet对人CD4^＋、CD8^＋T淋巴细胞亚群IFN-γ产生的调控作用。与对照组相比,转染后的人CD4^＋、CD8^＋T淋巴细胞t-betmRNA表达水平明显下降;转染siRNA后,CD4＋T淋巴细胞中IFN-γ＋细胞比例为（18.46±6.86）%,与对照组（50.20±5.91）%比较有显著性差异（P〈0.01）;CD8＋T淋巴细胞IFN-γ＋细胞比例为（74.18±9.33）%,和对照组（76.51±6.49）%比较差异不明显（P〉0.05）。体外转录合成的siRNA可有效降低人CD4^＋、CD8^＋T淋巴细胞t-bet的基因表达;转录因子t-bet对人不同淋巴细胞亚群IFN-γ的产生所起作用不同。     

生殖器疱疹初发患者外周血淋巴细胞检测结果分析

目的检测生殖器疱疹初发患者（GH）外周血T淋巴细胞亚群、NK细胞和B细胞的表达水平,探讨其发病机制与细胞免疫功能之间的关系。方法应用流式细胞仪检测20例初发生殖器疱疹患者外周血T淋巴细胞亚群、NK细胞和B细胞的表达水平,并与60例复发性生殖器疱疹患者（RGH）、35例健康对照者外周血检测结果相比较。结果（1）初发组和对照组相比,除NK细胞降低差异有显著性外,其他差异无显著性;（2）初发组与复发组相比,初发组T细胞、CD4^＋细胞、CD4^＋／CD8^＋均高于复发组,CD8^＋细胞百分比低于后者,差异有显著性;B细胞、NK细胞比例差异无显著性;（3）复发组与对照组相比,外周血中T细胞、CD4^＋细胞、NK细胞所占比例,CD4^＋／CD8^＋均降低,差异有显著性;CD8^＋细胞百分比升高,差异有显著性;B细胞比例差异无显著性。结论生殖器疱疹初发患者存在细胞免疫功能异常。     

In vivo induced allo-reactive natural killer cells.

We have previously shown that rat allo-selective cells of the CD2+CD5- phenotype were generated in Brown Norway (BN) rats after immunization with allogeneic Wistar/Furth (WF) cells, whereas immunization with semi-allogeneic F1 (WF/BN) cells generated CD2+CD5+ effector T cells. We now report that the allo-selective CD2+CD5- lymphocytes lacked expression of intact CD3 complexes and expressed NKR-P1 molecules although lower as compared to classical NK cells, implicating that these lymphocytes constitute a subset of NK cells. The CD5+ T cells were not cytolytically active in BN rats immunized with WF cells indicating an intersubset regulation with mutually exclusive activation of either allo-selective T cells or allo-selective NK cells. Cold target inhibition showed that lysis of both allogeneic target cells and NK-sensitive target cells was mediated by the same NKR-P1 intermediate effector cells. These NK cells lysed WF but not allogeneic Fischer 344 or autologous BN target cells, indicating selective recognition of an allogeneic determinant. Semiallogeneic F1 (WF/BN) target cells were not lysed. Furthermore, target cells from F1 (WF/BN) x WF back-cross hybrids lacking expression of RT1n (self-MHC class I) were susceptible to lysis, whereas back-cross hybrids expressing RT1n were protected from lysis, indicating that self-MHC molecules conferred protection from lysis. These findings implicate the existence of NKR-P1intermediate and NKR-P1high NK cell subsets with different regulation and function in vivo.     

TheRT1.G locus in the rat encodes a Qa/TL-like antigen

A new antigenic system in the rat homologous to theQa/TL antigen system in the mouse has been characterized. It was detected by antibodies raised in donor-recipient combinations that were matched for theRT1. A, B, D, E loci in the major histocompatibility complex (MHC): (R11×BN)F₁ anti-BN.1L(LEW), (R18×BN)F₁ anti-BN.1L, and BN.1LV1(F344) anti-BN.1L. Absorption analyses using these antisera and a variety of inbred, congenic and recombinant strains identified three alleles,RT1.G ^a ,G ^b ,G ^c , of whichG ^c is a null allele. The strain distribution of these alleles was determined, using 37 strains of rats representative of all of the prototypic haplotypes and a number of congenic and recombinant strains. The use of the congenic and recombinant strains showed that theRT1.G locus was linked to the MHC and that the most probable gene order wasA-E-G. Testcross analysis showed that the map distance betweenA andG was 1.4 cM(4/285 recombinants). The RT1.G antigen has a heavy chain ofM _r 46 000 and is present on both T and B cells.     

Dose-dependent recruitment of CD25+ and CD26+ T cells in a novel F344 rat model of asthma

The ovalbumin (OVA)-induced airway inflammation in rats is a commonly used model to explore the pathobiology of asthma. However, its susceptibility varies greatly between rat strains, and presently Brown Norway (BN) rats are preferentially used. Since recruitment of T cells to the lungs depends on the CD26 (dipeptidyl peptidase IV, DPPIV) expression, Fischer 344 strain (F344) rats are a highly relevant rat strain, in particular because CD26-deficient substrains are available. To establish a F344 rat model of asthma, we challenged F344 rats using different doses of aerosolized antigen (0%, 1%, 2.5%, 5%, and 7.5% OVA) and compared these effects with intratracheal instillation of OVA (1.5 mg/0.3 ml). Asthmoid responsiveness was determined by analysis of early airway responsiveness (EAR), antigen-specific IgE levels, as well as airway inflammation including the composition of T cell subpopulations in the bronchoalveolar lavage (BAL) and lung tissue with special respect to the T cell activation markers CD25 and CD26. Even low allergen doses caused allergen-specific EAR and increases of antigen-specific IgE levels. However, EAR and IgE levels did not increase dose dependently. Higher concentrations of OVA led to a dose-dependent increase of several immunological markers of allergic asthma including an influx of eosinophils, T cells, and dendritic cells. Interestingly, a dose-dependent increase of CD4(+)/CD25(+)/CD26(+) T cells was found in the lungs. Summarizing, we established a novel F344 rat model of aerosolized OVA-induced asthma. Thereby, we found a dose-dependent recruitment of cellular markers of allergic asthma including the activated CD4(+)/CD25(+)/CD26(+) T cell subpopulation, which has not been described in asthma yet.     

A polymorphism of the rat T-cell receptor β-chain variable gene 13 (BV13S1) correlates with the frequency of BV13S1-positive CD4 cells

Three rat BV13S1 alleles (T-cell receptor β-chain variable gene 13) were characterized by new BV13S1-allele specific monoclonal antibodies (18B1 and 17D5) and sequence analysis of expressed and genomic BV13S1. Two alleles were functional and designated BV13S1A1 present in strains LEW, BUF, PVG, and BV13S1A2 present in BN and WF. Their products differed by six amino acids, two of them in complementarity-determing region (CDR)1 and one in CDR2. A third nonfunctional allele, BV13S1A3P, was found in strains F344 and DA. Apart from a single nucleotide insertion, it was identical to BV13S1A2. All 12 rat strains tested showed association of TCRBC1 with BV8S2/4 alleles but not with the BV13S1 alleles, which may reflect a different gene order of the rat BV compared to mouse. BV13S1A1-encoded T-cell receptors (TCRs) which bind both monoclonal antibody (mAb) 18B1 and mAb 17D5 are over-represented in the CD4 lymphocyte subset. BV13S1A2-encoded TCRs which are stained by mAb 18B1 but not by mAb 17D5 show a slight CD8-biased expression. Preferential usage of BV13S1A1-positive TCRs by CD4 but not by CD8 cells in (LEW×WF)F1 hybrids and cosegregation of BV13SA1 and increased frequency of BV13S1 TCR-positive CD4 cells in a (LEW×BN)×BN backcross suggest structural differences of the two allelic products as the reason for their contrasting CD4/CD8 subset bias. Received: 6 October 1999 / Revised: 25 November 1999     

Proliferation and differentiation of alloselective NK cells after alloimmunization-evidence for an adaptive NK response.

We have previously demonstrated the activation of NK cells exhibiting RT1 allele-specific cytolytic activity following intraperitoneal immunization of certain rat strains with allogeneic cells. In the present study, we show that the NK allocytolytic activity in BN (RT1(n)) rats immunized with WF (RT1(u)) cells was associated with an increased proportion of peritoneal, as well as splenic, NK cells. Furthermore, the proliferation of NK cells was substantially increased in BN (RT1(n)) rats immunized with WF (RT1(u)) cells when compared to that in naive BN rats. In addition, the NK subpopulation exhibiting the allocytolytic activity in alloimmunized rats exhibited a decreased expression of the NKR-P1 and L-selectin molecules, but an increased expression of the LFA-1 molecule when compared to NK cells from naive rats. Thus, we have shown that the existence of peritoneal NK cells, exhibiting selective allocytolytic activity in alloimmunized rats, is probably due to a combination of RT1 allele-selective recruitment, proliferation, and the differentiation of NK cells. Therefore, in the same way that we regard T cells as being capable of adapting the immune response, this study presents evidence for the hypothesis that the specific cytolytic response of alloreactive NK cells should also be regarded as adaptive.     

IL-12 reduces the severity of Sendai virus-induced bronchiolar inflammation and remodeling

The goal of this research was to determine whether differential pulmonary IL-12 gene expression controls susceptibility to Sendai virus-induced chronic airway inflammation and fibrosis in inbred rat strains. Sendai virus-resistant F344 rats and susceptible BN rats were studied from 1 to 14 days following virus inoculation. F344 rats had 3.4-fold higher IL-12 mRNA levels detected by real-time PCR in lung than BN rats as early as two days following inoculation. This increase in mRNA was associated at two days with increased total IL-12 protein and with a 2-fold increase in numbers of bronchiolar, OX-6-positive dendritic cells and an increased number of IL-12 p40-positive, bronchiolar macrophages and dendritic cells (p<0.05). Virus-susceptible BN rats treated with 3 mug of recombinant, mouse IL-12 intraperitoneally at the time of virus inoculation had a 22.1% decrease in severity of chronic bronchiolar inflammation and a 23.8% decrease in fibrosis compared to virus-inoculated BN rats treated with saline. IL-12 treatment induced increased IFN-gamma mRNA and protein expression after virus inoculation (p<0.05). The results demonstrate that there is differential pulmonary IL-12 gene expression between virus-susceptible and resistant rat strains and that IL-12 treatment can provide significant protection from virus-induced chronic airway inflammation and remodeling during early life.     

Role of non-RT1 genes in the response of rat lymphocytes to Mycoplasma arthritidis T cell mitogen, concanavalin A and phytohemagglutinin

A comparison of splenic cells from various inbred rat strains indicated that DA, Lewis, Buffalo, August, Wistar Furth, and (LEW X BN)F1 all responded well to the Mycoplasma arthritidis T cell mitogen, phytohemagglutinin and concanavalin A, but cells from BN and MAXX rats were very weakly or nonresponsive. Cells from congenic strains expressing nonresponder background genes, and responder haplotypes at RT1 (BN.1L(LEW), RT1; BN.1A(DA), RT1av1) failed to respond significantly to the mitogens. Rats expressing responder background genes but the nonresponder haplotype at RT1 at RT1 (WF.1N-(MAXX), RT1n) exhibited high responses to all mitogens. The controlling role of non-RT1 genes was confirmed by testing tissue-typed (DA X BN)F2 progeny and (DA X BN)F1 X DA and (DA X BN)F1 X BN progeny. No association was seen between the expression of a/a, a/n, or n/n at RT1 and the degree of response to the mitogens. In contrast, as the proportion of DA non-RT1 genes increased, so did the degree of mitogenic responsiveness. Similar results were obtained by using a partially purified preparation of the mycoplasma T cell mitogen. The results indicated that in the (DA X BN)F1 hybrids, responsiveness to all mitogens was recessive: this contrasts with the (LEW X BN)F1 hybrids in which responsiveness was dominant. Finally, we showed that both responder and nonresponder splenic cells were capable of binding the M. arthritidis mitogen. The data contrast with those obtained with nonresponder mouse strains the cells of which failed to bind mitogen due to the absence of the E alpha chain of the I-E-coded molecule.     

Early high expression of IP-10 in F344 rats resistant to Sendai virus-induced airway injury

Weanling F344 and BN rats differ markedly in their susceptibility to Sendai virus-induced airway injury. Early gene expression that controls their differences in susceptibility remains poorly understood. In this study we combined suppressive subtractive hybridization and cDNA library array hybridization to identify genes differentially expressed in virus-susceptible BN and virus-resistant F344 rats during the first 3 days after inoculation. Differential expression of selected clones was further verified by quantitative RT-PCR. Seven virus-induced gene segments were identified. Of them, interferon-gamma-inducible protein 10 (IP-10), Mx1, and guanylate-binding protein-2 mRNA abundance in infected F344 rats was 201.5, 188.2, and 281.7% higher, respectively, than that of infected BN rats at 2 days after inoculation. In situ hybridization indicated that virus-induced IP-10 was expressed mainly in airway epithelial cells of F344 rats. Sendai virus infection can directly induce IP-10 expression in rat tracheal epithelial cells in vitro. IP-10 early high expression might contribute to the resistance to virus-induced airway disease in F344 rats by promoting Th1 responses and increasing antiviral activity.     

Genetic control of the development of experimental allergic encephalomyelitis in rats. Separation of MHC and non-MHC gene effects

Experimental allergic encephalomyelitis (EAE)-susceptible Lew and EAE-resistant Brown Norway (BN) rats and the corresponding MHC congenic strains were examined for their ability to develop clinical and histologic EAE. The ability of T cells from these animals to proliferate in vitro in response to whole guinea pig (GP) myelin basic protein (MBP), rat MBP, and to the major encephalitogenic peptide of GP MBP 66-88 (GP 68-88) was also assessed. We found that Lewis (Lew) was highly susceptible and showed good T cell responses to GP, MBP, rat MBP, and GP 68-88. Lew.1N (BN MHC on Lew background) and BN were not susceptible and T cells from these strains showed significant responses to GP MBP, but not to rat MBP or GP 68-88. Although BN.B1 (Lew MHC on BN background) was not susceptible to actively induced EAE, MBP-specific Lew T cells could transfer severe disease to BN.B1. BN.B1 T cells showed responses to GP-MBP, rat MBP, and GP 68-88 and, when transferred to naive BN.B1 or Lew, induced only mild clinical EAE in both strains. Increasing the number of T cells from BN.B1 had no effect on the severity of clinical symptoms in either recipient, suggesting some deficiency in the T cell repertoire that is necessary for induction of severe EAE. These results suggest that 1) the T cell response to rat MBP and GP68-88 (but not to sites other than 68-88 in GP MBP) is necessary for susceptibility to EAE; 2) the ability to respond to both rat MBP and GP 68-88 is determined by the MHC gene products on APC; and 3) given a permissive MHC, the T cell response that results in EAE is influenced by non-MHC genes.