Neuronal apoptosis and neurofilament protein expression in the lateral geniculate body of cats following acute optic nerve injuries

The visual pathway have 6 parts, involving optic nerve, optic chiasm, optic tract, lateral geniculate body, optic radiation and cortical striatum area. Corresponding changes may be found in these 6 parts following optic nerve injury. At present, studies mainly focus on optic nerve and retina, but studies on lateral geniculate body are few. OBJECTIVE： To prepare models of acute optic nerve injury for observing the changes of neurons in lateral geniculate body, expression of neurofilament protein at different time after injury and cell apoptosis under the optical microscope, and for investigating the changes of neurons in lateral geniculate body following acute optic nerve injury. DESIGN： Completely randomized grouping design, controlled animal experiment. SETTING： Department of Neurosurgery, General Hospital of Ji＇nan Military Area Command of Chinese PLA. MATERIALS： Twenty-eight adult healthy cats of either gender and common grade, weighing from 2.0 to 3.5 kg, were provided by the Animal Experimental Center of Fudan University. The involved cats were divided into 2 groups according to table of random digit： normal control group （n=3） and model group （n=25）. Injury 6 hours, l, 3, 7 and 14 days five time points were set in model group for later observation, 5 cats at each time point. TUNEL kit （Bohringer-Mannheim company ）and NF200＆ Mr 68 000 mouse monoclonal antibody （NeoMarkers Company） were used in this experiment. METHODS： This experiment was carded out in the Department of Neurosurgery, General Hospital of Ji＇nan Military Area Command of Chinese PLA between June 2004 and June 2005.① The cats of model group were developed into cat models of acute intracranial optic nerve injury as follows： The anesthetized cats were placed in lateral position. By imitating operation to human, pterion approach was used. An incision was made at the joint line between outer canthus and tragus, and deepened along cranial base until white optic nerve via optic nerve pore and further to brain tissue. Optic nerve about 3 mm was liberated and occluded by noninvasive vascular clamp for 20 s. After removal of noninvasive vascular clamp, the area compressed by optic nerve was hollowed and narrowed, but non-fractured. Skull was closed when haemorrhage was not found. Bilateral pupillary size, direct and indirect light reflect were observed. Operative side pupil was enlarged as compared with opposite side, direct light reflect disappeared and indirect light reflect existed, which indicated that the models were successful. Animals of control group were not modeled .② The animals in the control group and model group were sacrificed before and 6 hours, 1, 3, 7 and 14 days after modeling respectively. Lateral geniculate body sample was taken and performed haematoxylin ＆ eosin staining. Immunohistochemical staining showed lateral geniculate body neurofilament protein expression, and a comparison of immunohistochemial staining results was made between experimental group and control group. Terminal deoxynucleo-tidyl transferase （TdT）-mediated dUTP-biotin nick end labeling （TUNEL） was used to label apoptotic cells in lateral geniculate body. MAIN OUTCOME MEASURES： Neuronal morphological change, neurofilament protein expression and cell apoptosis in lateral geniculate body following acute optic nerve injury. RESULTS： Twenty-eight involved cats entered the final analysis. ① Histological observation results： In the control group, cell processes were obviously found, which were few or shortening in the model group. ② Neuronal neurofilament protein expression： Cells in lateral geniculate body in the control group and at 6 hours after injury presented clear strip-shaped staining, and those at 7 and 14 days presented irregular distribution without layers and obviously decreasing staining intensity. The positive rate of neurofilament protein in lateral geniculate body in control group and 6 hours, l, 3, 7 and 14 days after injury was （ 10.22±0.42） %, （10.03±0.24） %, （9.94±0.14） %, （9.98±0.22） %, （8.18±0.34） % and （6.37±0.18）%, respectively. Positive rate of neurofilament protein in control group, at 6 hours, 1 or 3 days after injury was significantly different from that at 7 days after injury （P 〈 0.05）; Positive rate of neurofilament protein in control group, at 6 hours, 1, 3 or 7 days after injury was significantly different from that at 14 days after injury （P 〈 0.05）. It indicated that neuronal injury in lateral geniculate body was not obvious within short term after optic nerve injury, but obvious at 7 days after injury and progressively aggravated until at 14 days after injury.③ Neuronal apoptosis： TUNEL staining showed that neuronal apoptosis in lateral geniculate body appeared at 7 days after injury, and a Lot of neuronal apoptosis in lateral geniculate body was found at 14 days after injury. It indicated that neuronal injury in lateral geniculate body was related to apoptosis. CONCLUSION： In short term after optic nerve injury （within 7 days）, nerve injury of lateral geniculate body is not obvious, then, it will aggravate with the elongation of injury time. The occurrence of neuronal iniury of lateral geniculate body is related to the apoptosis of nerve cells.

MRI Evaluation of Lateral Geniculate Body in Normal Aging Brain Using Quantitative Susceptibility Mapping

Objective To investigate the changes of lateral geniculate body(LGB) in the normal aging brain using quantitative susceptibility mapping(QSM) technique. Methods Magnetic resonance(MR) phase and magnitude images were acquired from enhanced gradient echo T2 star weighted angiography sequence with 16 echoes on 3.0T MR system using the head coil with 32 channels. Morphology Enabled Dipole Inversion(MEDI) method was applied for QSM, and the susceptibility value of LGB was measured by region of interest(ROI) drawn manually on three orthogonal planes. Results LGB of the middle-aged group had a higher susceptibility value(0.16±0.05 ppm) than that of the youth group(0.12±0.05 ppm) and elderly group(0.13±0.03 ppm)(all P<0.05). Partial correlation analysis demonstrated that there was significantly positive correlation between susceptibility value and age in the youth group(r=0.71, P<0.05). Conclusion LGB could clearly be identified on QSM in the brain in vivo.

Heat shock protein 72 confers protection in retinal ganglion cells and lateral geniculate nucleus neurons via blockade of the SAPK/JNK pathway in a chronic ocular-hypertensive rat model

Optic nerve transection increased the expression of heat shock protein 72 （HSP72） in the lateral geniculate body, indicating that this protein is involved in the prevention of neuronal injury. Zinc sulfate and quercetin induced and inhibited the expression of HSP72, respectively. Intraperitoneal injections of zinc sulfate, SP600125 （c-Jun N-terminal kinase inhibitor）, or quercetin were performed on retinal ganglion cells in a Wistar rat model of chronic ocular hypertension. Our results showed that compared with the control group, the expression of HSP72 in retinal ganglion cells and the lateral geniculate body was increased after the injection of zinc sulfate, but was decreased after the injection of quercetin. The expression of phosphorylated c-Jun N-terminal kinases and phosphorylated c-Jun were visible 3 days after injection in the control group, and reached apeak at 7 days. Zinc sulfate and SP600125 significantly decreased the expression of p-c-Jun, whereas quercetin significantly enhanced the expression of this protein. These results suggest that HSP72 protects retinal ganglion cells and lateral geniculate body in a rat model of chronic ocular hypertension from injury by blocking the activation of the stress-activated kinase/c-Jun N-terminal kinase apoptotic pathway.

磁共振DTI及DTT技术在成人视放射病变中的初步临床应用

目的应用磁共振弥散张量成像(DTI)及弥散张量纤维束成像(DTT)技术评估成人视放射病变的各向异性程度、视放射神经纤维束构象特征及临床价值及探讨视放射病变对外侧膝状体(LGN)形态学的影响。方法收集经磁共振检查、临床资料或手术病理证实累及视放射的脑内病变12例及磁共振检查无异常的健康体检者12例,以上受检者均进行过磁共振DTI及DUALTSE序列扫描。根据是视放射是否受累及,将12对视放射分成病变组、对照组,通过后处理软件分别获得部分各项异性指数(FA)值、表观弥散系数(ADC)值、平均纤维束长度(ML)、单位像素纤维束数目(MF)、LGN的高度与体积及进行纤维束追踪与成像分析,且两两比较进行统计学分析。结果12例病例中有16个视放射纤维束表现为不同程度的纤维束稀疏、移位或破坏,累及视放射的病变可导致LGN大小、形态甚至信号发生一定改变,且病例组与健康组比较具有统计学差异性,其ADC值、ML值及MF值均较健康组有所升高,但差异无统计学意义,病变组与对照组间各指标比较均无统计学意义。累及视放射的病变可导致LGN形态或信号发生一定改变,病例组LGN高度及体积的缩小与健康组比较具有统计学差异性。结论DTI及DTT技术可作为评价颞、枕部病变所致视放射及LGN形态、功能改变的既安全又客观指标;术前运用DTT技术对保护具有重要功能的白质纤维束及了解病变与该纤维束之间的关系具有重要临床意义。

后丘脑动脉的显微解剖及其微血管构筑

用手术显微镜观测了48侧成人后丘脑的动脉,并用墨汁明胶灌注、厚片透明、碱性磷酸酶染色示血管内皮及甲酯铸型法,在体视显微镜和扫描电镜下观察了14侧胎儿后丘脑的微血管构筑.后丘脑的动脉分为内侧膝状体丘脑动脉、外侧膝状体丘脑动脉和膝状体间丘脑动脉.前两者中的小支分布到内、外侧膝状体,较大支及膝状体间丘脑动脉主要分布至丘脑枕中、上部.外侧膝状体微血管呈疏密相间排列,内侧膝状体毛细血管网致密,无分层现象.后丘脑微血管铸型的表面特征与丘脑相类似,微动脉多呈锐角分支,微静脉单独走行或几条微动脉围绕一条微静脉.可见毛细血管吻合和毛细血管前吻合.

视觉传导路营养动脉的显微解剖及其临床意义

目的研究视神经、视交叉、视束、外侧膝状体等结构的动脉,为视力障碍和血管造影提供基础资料。方法手术显微镜下对100侧成人脑的视神经、视交叉、视束、外侧膝状体的动脉进行显微解剖观察,并做病理组织学研究。结果视神经呈分段分层供血;视交叉中央区微血管稀少;视束的后半部由脉络丛前动脉供血;外侧膝状体的血供为多来源而前外侧为单来源供血。50～70岁60侧脑标本的来源动脉88.3%有动脉硬化改变。结论视神经和视交叉中央部、视束后半部及外侧膝状体的前外侧为血供的危险区;是视野缺损的病因之一。

剥夺性弱视猫外侧膝状体c-fos基因及Fos蛋白表达

为研究生后关键期内,正常猫及剥夺性弱视猫外侧膝状体神经元功能形态的变化规律,对正常视发育敏感期的幼猫行左眼睑缝合术,造成剥夺性弱视模型,采用Nissl染色法及电镜观察正常猫及剥夺性弱视猫外侧膝状体神经元的形态改变,并用免疫组化和原位杂交技术检测Fos蛋白及cfos基因的表达情况。结果显示:(1)剥夺猫剥夺层外侧膝状体神经元的截面积比非剥夺层及正常猫的明显变小,差异有显著性(P<0.05);(2)超微结构显示:剥夺性弱视猫的剥夺层出现大量变性的细胞,剥夺4周时最为显著;(3)正常猫外侧膝状体神经元Fos蛋白和cfos原位杂交的阳性细胞数及OD值随着时间的延长而降低。同龄猫剥夺层外侧膝状体Fos蛋白和cfos原位杂交阳性细胞数及OD值较正常猫减少(P<0.05)。结果提示:猫视觉的可塑性敏感期为生后4周到8周。剥夺性弱视猫外侧膝状体剥夺层及非剥夺层神经元形态及功能与正常猫相比较均发生改变。Fos法可以成为衡量弱视猫外侧膝状体兴奋性状态与形态学定位相结合的实验方法,但必须注意神经可塑性对其的影响。

单眼视功能损害的原发性开角型青光眼患者的外侧膝状体损伤

目的研究单眼晚期视功能损害的原发性开角型青光眼患者外侧膝状体的形态改变情况。方法选取单眼晚期视功能损害的原发性开角型青光眼患者6例(青光眼组)及性别、年龄匹配的正常对照者8例(对照组),均行外侧膝状体的3.0T磁共振成像扫描,测量外侧膝状体的最大高径和体积。比较青光眼组及对照组杯盘比、视网膜神经纤维层(retinalnervefiberlayer,RNFL)厚度、视野平均缺损值及对比分析青光眼组及对照组外侧膝状体各相关指标的统计学差异。结果所有受试者外侧膝状体均可清晰成像。青光眼组右侧外侧膝状体最大高径、体积分别为(4.52±0.57)mm、(104.80±21.10)mm3,左侧为(4.30±0.26)mm、(101.50±27.70)mm3,差异均无统计学意义(t=0.850,P=0.415;t=0.235,P=0.819)。正常对照组右侧外侧膝状体最大高径、体积分别为(5.14±0.35)mm、(136.80±14.40)mm3,左侧为(4.98±0.31)mm、(141.90±16.80)mm3,差异均无统计学意义(t=0.665,P=0.510;t=0.141,P=0.888)。青光眼组双侧外侧膝状体最大高径及体积均较正常对照组减小(均为P<0.05);杯盘比、RNFL厚度差异有显著统计学意义(均为P<0.001),而视野平均缺损值差异无统计学意义(P=0.143)。结论原发性开角型青光眼单眼视功能损害的患者中枢损伤可累及双侧外侧膝状体,二维最大高径及三维体积均明显萎缩,3.0T磁共振成像可以清晰显示这个变化,从影像学角度加深对青光眼中枢损伤的认识。

小鼠外侧膝状体主要蛋白的蛋白组学鉴定

目的:用蛋白组学鉴定小鼠外侧膝状体内的主要蛋白。方法:提取小鼠外侧膝状体的蛋白质,通过二维凝胶电泳分离蛋白,用PDQuest图像分析软件选择电泳图谱中的高含量蛋白,用MALDI TOF/TOF串联质谱仪分析蛋白质,所得的质谱图通过GPS软件在Mascot数据库中检索并鉴定蛋白质,并用Western-blotting进一步验证鉴定的蛋白。结果:在小鼠外侧膝状体共鉴定了33种主要蛋白,其中结构蛋白5种,代谢酶21种,转运蛋白3种,信号转导蛋白2种,应激蛋白1种,未命名蛋白1种。Western-blotting验证的蛋白与质谱仪鉴定的结果一致。结论:本结果为该区域蛋白质的研究提供实验资料。

金黄仓鼠视皮层、上丘和外侧膝状体中的血管活性肠肽(VIP)神经元及其纤维

用程序稍有不同的两种ＰＡＰ法对视觉通路中的三个重要区域视皮层、上６和外侧膝状体中的 血管活性肠肽（ＶＩＰ）进行了定位，．视皮层Ⅱ至Ⅵ层都有ＶＩＰ阳性神经元分布，内域性的阳性神经 纤维遍布整个视皮层。上丘中的ＶＩＰ阳性神经无数量较少，主要分布于上丘的咀部表层，视皮层和 上丘中的ＶＩＰ神经元均为非锥体型的多极和双极神经元。外侧膝状体中未发现有ＶＩＰ阳性神经元 胞体．只有弥散的阳性神经纤维。

糖尿病大鼠脑外侧膝状体神经元退行性变及APP17肽的作用

目的 通过观察糖尿病大鼠外侧膝状体神经元超微结构改变和神经元内凋亡相关因子Bax、Bcl-2、Cyto C的表达,证实糖尿病大鼠是否存在脑内视觉传导通路外侧膝状体神经元退行性改变,APP17肽对其是否有改善作用。方法 用链脲佐菌素(STZ)腹腔注射诱发糖尿病模型,10周后取脑组织行Bax、Bcl-2、Cyto C的免疫组化染色,同时取外侧膝状体处脑组织作电镜观察。结果 糖尿病组外侧膝状体腹侧核内Bax、Cyto C阳性反应神经元数目多、染色深,Bcl-2三组间无明显差异,APP17肽治疗组的Bax、Bcl-2、Cyto C的表达接近正常组。超微结构发现糖尿病组神经元有固缩、核膜凹陷、线粒体肿胀等退行性变,给予APP17肽后上述改变明显好转。结论 糖尿病大鼠发生了外侧膝状体神经元的退行性改变,神经元可能处于凋亡前状态;APP17肽可改善糖尿病大鼠外侧膝状体神经元的退行性改变。

人外侧膝状体的血液供应及其临床意义

目的:为外侧膝状体(LGB)缺血所致的视野缺损提供形态学依据。方法:手术显微镜下观察成人和胎儿脑的LGB动脉的来源和微血管构筑,部分脑标本用组织切片方法观察营养LGB动脉的粥样硬化病理改变。结果:LGB营养动脉第一级来自颈内动脉和大脑后动脉,二级为脉络丛前动脉、脉络丛后外动脉和丘脑膝状体动脉,三级构成LGB的小动脉。50岁以上的标本,LGB 的一、二级动脉有硬化改变的占88%,二级小动脉被阻塞占10%。结论:二级动脉在LGB内有各自的供血区,脉络丛前动脉是供应IGB前部和外侧部的唯一动脉,大脑后动脉营养LGB的其余部分。不同动脉的阻塞可导致不同种类的视野改变,是视野缺损的原因之一。

幼儿外侧膝状体及视皮质微血管的形态学

目的:探讨幼儿外侧膝状体及视皮质微血管构筑的形态结构。方法:采用8例幼儿外侧膝状体及视皮质,经碱性磷酸酶染色,组织切片,光镜观察。结果:幼儿视皮质(17区)后1/3的微血管密度最高,前1/3次之,中1/3最低。外侧膝状体后2/3的微血管密度高于前1/3。视皮质内动脉多数以直角、少数以锐角发自软脑膜动脉。视皮质内静脉数量明显少于动脉。静脉属支汇入处可见一三角形膨大,且深层微静脉粗,浅层微静脉细。结论:幼儿外侧膝状体及视皮质相对应区域微血管同步发育。皮质微静脉的这种结构特点可能是皮质微静脉栓塞的因素之一。

刺激兔杏仁体影响内膝体听觉神经元的ON-OFF反应

在２３只三碘季铵酚麻痹的新西兰兔上记录细胞外放电，观察短纯音诱发的内膝体神经元ｏｎｏｆ反应的特性及电刺激边缘系统杏仁外侧核（Ｌａｔｅｒａｌａｍｙｇｄａｌｏｉｄｎｕｃｌｅｕｓ，ＬＡｍ）对反应的影响。实验发现，内膝体神经元的ｏｎｏｆ反应与纯音刺激的强度、频率及作用时程有关；刺激ＬＡｍ，可以抑制ｏｎｏｆ反应，或是使ｏｎｏｆ反应放电构型发生变化。ｏｎｏｆ反应是神经元对声音信号作用时程及声音的起止进行编码的方式之一，ＬＡｍ对ｏｎｏｆ反应的影响表明，边缘系统杏仁体的活动可以调控听觉中枢对声音时间信息的编码。

补精益视片对SD大鼠慢性高眼压模型外侧膝状体尼氏小体的影响

目的观察补精益视片对慢性高眼压模型(elevatedintraocularpressureEIOP)大鼠外侧膝状体中尼氏小体(nisslbody)含量的影响,探讨补精益视片视功能保护的作用机理。方法选取30只SD大鼠,随机分为对照组、给药组及模型组,每组各10只。采用烙闭巩膜上静脉方法制作慢性高眼压大鼠动物模型,每组连续灌胃8周后处死大鼠,观察补精益视片对EIOP大鼠眼压、外侧膝状体(lateralgeniculatenucleusLGN)尼氏小体含量的影响。结果相比造模前,从造模即刻开始至造模后8周,给药组及模型组大鼠的眼压均有明显升高,差异具有统计学意义(均P<0.01);造模后8周与造模即刻相比,给药组眼压有降低趋势,差异有统计学意义(P<0.01),而模型组眼压无降低趋势;模型组尼氏小体总面积(55863.31±18427.166S/μm2)及积分光密度(16084.76±6013.412)较对照组(114533.71±17849.482S/μm2,35237.50±4626.313)及给药组(108020.95±27719.546S/μm2,31261.33±7800.446)明显偏低,差异具有统计学意义(均P<0.01),给药组尼氏小体总面积及积分光密度较对照组稍偏低,差异无统计学意义(P>0.05)。结论补精益视片能提高慢性EIOP模型大鼠LGN尼氏小体含量,从而发挥视功能保护作用。

金黄地鼠上丘和外侧膝状体之间的联系

本实验采用了顺行和逆行追踪技术,对金黄地鼠上丘与丘脑视核团的纤维联系进行了实验观察。一、用尼氏和Loyez染色法,对4只正常金黄地鼠上丘和外侧膝状体背核和腹核的正常结构做了观察。二、^(3)H-亮氨酸和^(3)H-脯氨酸注入动物上丘不同部位(4只,存活期一天)后,可见神经末梢标记于同侧的外侧膝状体背核和腹核的外侧部位。若注射部位在上丘外侧,其投射部位在外侧膝状体背核和腹核的尾外侧;注射部位移向内侧,投射部位移向吻外侧。三、将HRP注入外侧膝状体背核(4只,存活期一天)或腹核(2只,存活期一天)或后外侧核(2只,存活期一天)后,在同侧上丘浅层见有标记神经元。在上丘深层则未见。本实验说明了上丘浅层的神经元对同侧的外侧膝状体背核和腹核有局部定位的投射,并按视野和视网膜将该投射作定位排列。

丰富环境对单眼剥夺小鼠视皮质与外侧膝状体Sortilin表达的影响

目的:探讨丰富环境(EE)对弱视小鼠初级视皮质和外侧膝状体Sortilin的表达影响。方法:选择36只21d昆明小鼠,雌雄不限,随机分为正常组(Control)、单眼剥夺+标准环境组(MD+SE)和单眼剥夺+丰富环境组(MD+EE),通过行为学检测各组小鼠视功能改变、免疫组织化学方法检测各组小鼠视皮质和外侧膝状体Sortilin的表达。结果:行为学结果显示:与Control组相比,MD+SE组探爪触地成功率明显降低(P<0.05),MD+EE组探爪触地成功率显著高于MD+SE组(P<0.05);免疫组织化学结果显示:与Control组相比,MD+SE组外侧膝状体背内侧Sortilin阳性神经元数目显著升高(P<0.001);MD+EE组显著低于MD+SE组,但高于Control组(P<0.001);与Control组相比,MD+SE组小鼠视皮质Sortilin阳性神经元数目显著降低(P<0.001);MD+EE组显著高于MD+SE组(P<0.001),但显著低于Control组(P<0.001)。结论:丰富环境改善弱视小鼠视功能可能通过调节视皮质和外侧膝状体Sortilin的表达实现。

一种脑启发式的边缘检测模型

边缘是物体的基础特征,传统边缘检测方法具有一定的局限性。鉴于人类视觉系统能高效准确地感知物体的边缘信息,根据大脑侧膝体(Lateral Geniculate Nucleus,LGN)和初级视皮层(primary visual cortex,V1)简单细胞的感受野特性,提出一种脑启发式的前馈LGN-V1(Feedforward LGN-V1,FLV)视觉感知模型。首先用高斯函数之差模拟单个LGN细胞的同心圆式感受野,再通过同类LGN细胞的联合构建细胞组,最后将两类细胞组分别共线排列并平行放置模拟得到特定偏好朝向V1简单细胞。通过多简单细胞响应的整合获取全体V1简单细胞的响应。实验结果表明,FLV模型能体现真实简单细胞的生物特性。较传统的边缘检测方法而言,所提模型效果更优,具有更好的鲁棒性。

单眼视觉剥夺猫外膝体神经元的双眼反应特性

采用在位（ｉｎ ｖｉｖｏ） 胞内记录技术，研究了单眼视觉剥夺猫外膝体（ＬＧＮ） 神经元的双眼反应特性（ｂｉｎｏｃｕｌａｒｉｔｙ） ， 结果发现单眼剥夺猫外膝体几乎所有的双眼反应神经元都对非优势眼的闪烁光斑刺激有不同程度的反应，并且剥夺层和非剥夺层神经元在反应特性上没有明显差异。但是，与非剥夺层神经元相比，几乎没有剥夺层的神经元能对非优势眼的正弦移动光栅刺激起反应，并受其空间频率的调制。结果提示皮层下外膝体水平上这种双眼反应的某些精细反应性质可能与后天视觉经验的修饰有关，并可能受皮层反馈输入的影响。

噪声和二硫化碳对大鼠外膝体神经元光反应的影响及其联合效应

目的:观察噪声或二硫化碳(CS2)暴露对大鼠外侧膝状体(LGB)神经元光反应的影响及二者的联合效应。方法:脉冲噪声刺激和光栅刺激由计算机控制输出,CS2通过皮下注射,运用电生理学方法记录LGB神经元电活动。结果:噪声暴露后有21%的神经元光反应被抑制,当噪声持续时,抑制程度有增强的趋势,呈现出剂量?效应关系。不同剂量的CS2暴露,神经元受到不同程度的抑制,亦呈剂量-效应关系。噪声和CS2同时作用时,呈一定的协同作用。结论:噪声或者CS2的单独作用可明显抑制外膝体神经元的光反应,在共同作用时存在联合效应,主要表现为协同效应。