Evidence for polyreactivity seen with monoclonal antibodies produced against type II collagen

Specific type II collagen monoclonal antibodies are needed for the quantification of articular cartilage collagen. In this study we produced and characterized 29 type II collagen monoclonal antibodies. Hybridomas were generated from mice immunized with rat type II collagen, selected for high antibody production against type II collagen using ELISA. Antibodies from selected and cloned hybridoma cells were purified by affinity chromatography and their reactivity tested by ELISA against a panel of antigens including actin, thyroglobulin, and single stranded DNA, all of which have been used to characterize the ‘naturally occurring antibodies’. It was found that many of the anti-type II collagen monoclonal antibodies reacted to more than one antigen. The monospecific antibodies had higher affinity to type II collagen than the antibodies which demonstrated multireactivity. Because of the prevalence of polyreactive anti-type II collagen antibodies, it is advisable to employ highly selective methodologies to isolate high affinity monospecific antibodies to type II collagen.     

Reconstruction of the basement membrane in a cultured submandibular gland

Summary In a rat submandibular rudiment on day 16, both laminin (LM) and type IV collagen (Col-IV) were found in all cases to colocalize not only in the basement membrane, but also in the rough endoplasmic reticulum of the epithelial cells, indicating that the synthesis of the components of basement membrane is greatly enhanced at this particular stage of extensive branch formation. Using the submandibular gland from a 16-day embryo, the model system was developed to determine the structural organization of the basement membrane. The pre-existing basement membrane was digested with collagenase and dispase, causing its complete disappearance. The subsequent gradual reconstruction of an authentic basement membrane was confirmed by electron microscopy and immunohistochemistry of LM and ColIV. In the model system, this recovery started at 4 h of culture, and formation was complete by 8 h. During the recovery, thick bundles of actin filaments appeared transitionally in the basal cytoplasm. Electron microscopic analysis indicated two precursor structures, aggregated fuzzy fibers (type 1 extracellular matrix (ECM)) and 10-nm-thick strand piles (type 2 ECM), and an authentic basement membrane structure appeared during the course of membrane reconstruction. LM and Col-IV were always located together in these three structures. These observations clearly indicate that the precursors, containing LM, Col-IV and most likely heparan sulfate proteoglycan, appeared to form immediately following their secretion into the extracellular space, and assembled into the rigid structure of basement membrane within 8 h. The ultrastructural and immunohistochemical process of basement membrane reconstruction appeared to coincide closely with that of the glomerular basement membrane in developing kidney. The three-stage assembly may therefore be a common process of basement membrane formation.     

Immunolocalization of type III collagen and procollagen in cirrhotic human liver using monoclonal antibodies

Summary Immunolocalization of type III collagen and procollagen in cirrhotic human liver was studied using monoclonal antibody specific for the helical determinant of type III collagen extracted from human placenta. Deparaffinized, trypsin-treated cirrhotic liver sections from 8 autopsy cases were examined by the unlabeled peroxidase-antiperoxidase and immunofluorescence techniques. These techniques revealed the localization of this epitope shared by type III collagen and procollagen not only in the extracellular matrix of hepatocytes and sinusoidal cells but also in the cytoplasm. In hepatocellular carcinoma concurrent with cirrhosis, neoplastic cells were shown to react with this antibody as well.These results are consistent with data obtained using antiserum specific for bovine type III procollagen aminopeptide which appeared in our previous report.     

抗血小板糖蛋白VI单克隆抗体的制备及其功能研究

目的:制备抗血小板糖蛋白VI(GPVI)单克隆抗体,观察其在体外抗血小板黏附和聚集功能。方法:采用基因重组技术体外表达血小板糖蛋白VI胞外区重组蛋白(rGPVI)。以rGPVI免疫小鼠,经细胞融合及筛选后制备抗GPVI单克隆抗体。采用血小板聚集实验观察该单抗对胶原、Convu lxin及ADP诱导的血小板聚集的影响;利用平行板流动小室技术研究在高剪切力条件下该单抗对血小板在胶原表面黏附的抑制效果。结果:正确构建了rGPVI表达载体pET-20b(+)-GPVI,rGPVI在原核细胞中有效表达。rGPVI能够被抗Penta-H is单抗和抗GPVI多抗识别。制备的抗GPVI单克隆抗体SZ118能够识别rGPVI,并与血小板有特异的结合能力。SZ118能明显抑制纤维状胶原和Convu lxin诱导的血小板聚集,呈抗体剂量依赖性;对ADP诱导的血小板聚集无明显影响。血小板黏附实验表明,SZ118能够明显阻断在高剪切力条件下血小板与纤维状胶原表面的黏附。结论:成功制备抗GPVI单克隆抗体SZ118,该抗体与血小板有良好的结合能力,显著抑制胶原诱导的血小板聚集并明显降低血小板与胶原的黏附反应。     

Immunohistochemical localization of myoepithelial cells and basement membrane in normal,benign and malignant human breast lesions

Summary Distributions of actin and type IV collagen were investigated immunohistochemically as markers for myoepithelial cells and basement membranes. Carnoy's and Methacarn-fixed, paraffin-embedded tissues from 103 human breast lesions from 103 patients were examined; 65 with carcinomas, 27 with mastopathies, 9 with fibroadenomas and 2 with phyllodes tumours. Fifty-five samples of the normal mammary gland tissue adjacent to tumours were also included for comparison. In normal breast and benign breast diseases, type IV collagen was identified around the mammary glandular cells and actin-positive cells were demonstrated to attach to basement membranes. In noninvasive carcinomas, type IV collagen was found as a continuous lining around a cell nest, while actin-positive cells were usually absent in ductal but quite numerous in lobular carcinomas. In invasive carcinomas, type IV collagen was fragmented or absent and actin-positive cells were very uncommon around the fragmentary basement membranes. These results suggest that the different distributions of myoepithelial cells and basement membrane material is useful in the differential diagnosis of surgical pathology of the breast.This work is supported in part by grant-in-aid for cancer research 62010025, from the Ministry of Education, Science and Culture, Japan     

Ultrastructure and development of a thick basement membrane-like layer in the anchoring villi of macaque placentas

Background: Anchoring villi and cytotrophoblastic cell columns are important structural components involved in placental morphogenesis. We have previously described the presence of an unusual basement membrane-like layer (BMLL) that separates these placental compartments. The purpose of the present study was to identify developmental changes in the ultrastructure of the BMLL and to assess its changes in extracellular matrix composition over the course of gestation. Methods: Conventional techniques were used to examine macaque placental tissue by transmission electron microscopy. Standard immunoperoxidase methods were used to identify type IV collagen, laminin and fibronectin in paraffin sections. Results: Until day 35 of gestation the BMLL was 70–100 nm thick and appeared similar to basement membranes seen in other regions of the villus, although it usually lacked a lamina lucida along the surface adjacent to the cytotrophoblast cells. Immunohistochemistry revealed the presence of laminin and type IV collagen in the BMLL. By 53 days of gestation the BMLL had hypertrophied at the junction of the anchoring villus and cell column, measuring 2,000–5,000 nm in thickness. The BMLL retained immunoreactivity for laminin and type IV collagen. Ultrastructural examination revealed the presence of a new component in the form of 10 nm microfibrils. By 89 days of gestation the BMLL was not reactive for laminin or type IV collagen but otherwise maintained the structural organization seen at 53 days. No additional changes were observed in the BMLL during late pregnancy. Conclusions: The BMLL is a distinct extracellular matrix region that separates the distal aspect of the anchoring villus from the proximal portion of the cell columns. Evidence indicates that adjacent cytotrophoblast plays a prominent role in the production of the BMLL. The BMLL may serve to organize this complex tissue by separating fetal mesenchyme from cytotrophoblast cells that are proliferating, differentiating, and migrating. Modifications to the composition of the BMLL may indicate changes in the role this matrix plays in the development of the placenta. © 1994 Wiley-Liss, Inc.     

Effects of ACE inhibition on the expression of type IV collagen and laminin in renal glomeruli in experimental diabetes

In the present study, we examined electron microscopically and immunohistochemically the effects of perindopril, an angiotensin-converting enzyme inhibitor, on renal microangiopathy in streptozotocin-induced diabetes in rats. To investigate changes in glomerular basement membrane (GBM) and tubular basement membrane components, we immunohistochemically localized type IV collagen and laminin. Animals have been divided into three groups of eight adult male rats each. The first group was the non-diabetic control group. The second group consisted of untreated diabetic rats. The third group consisted of diabetic rats that were treated with perindopril for 6 weeks. Blood glucose levels and body weight were measured. Morphometric analysis of kidney tissue was performed using light and electron microscopy to quantify glomerular size and thickness of the GBM. Blood glucose levels in diabetic rats were significantly increased when compared with non-diabetic controls. Blood glucose levels were not affected by perindopril treatment. Untreated diabetic rats showed increased glomerular size, thickening of the GBM and an increase in mesangial matrix as compared with controls. Treatment with perindopril prevented effectively glomerular hypertrophy and thickening of the GBM. Significant increase in type IV collagen and laminin was found in thickened GBM and mesangial matrix in kidneys of untreated diabetic rats. In perindopril-treated diabetic rats, staining of type IV collagen and laminin was less strong when compared with untreated diabetic rats. In conclusion, our data suggest that perindopril treatment is effective in preventing renal lesions possibly by ameliorating the diabetes-induced increase in expression of type IV collagen and laminin.     

Distribution of basement membrane laminin and type IV collagen in human reactive lymph nodes

The location of two basement membrane components, laminin and the 7-S domain of type IV collagen, was studied in human lymph nodes using the peroxidase-antiperoxidase method. Basement membrane antigens were present on the walls of blood vessels and of marginal, trabecular and medullary sinuses. Thin, fragmented fibre-like staining was present also in parenchyma outside the germinal centres, in a pattern overlapping with reticular fibres as seen on conventional reticulin stains. This finding suggests that basement membrane components are a part of the reticular fibres of lymph nodes, or are closely associated with them.     

Expression of type VII collagen,the major anchoring fibril component,in normal and neoplastic human nervous system

The distribution of type VII collagen was examined in the normal human nervous system, in brain tumour biopsies and in glioma cell lines by immunohistochemistry and western blotting. In normal tissue, positivity was observed beneath choroid plexus epithelial cells and around pineal gland and pituitary gland cell nests, while other brain regions and peripheral nerves were negative. Expression was preserved in most related tumours (choroid plexus papilloma, pineoblastoma, pituitary adenoma). Scattered abnormal vessels showed neoexpression of type VII collagen in about half of the astrocytic and ependymal tumours. Glioma cells in situ were consistently negative for type VII collagen, where-as the glioblastoma cell lines were positive. Our results suggest that anchoring fibrils or at least epitopes of their major structural component are present in normal and pathological cerebral structures, indicating a unique distribution of type VII collagen in the nervous system.     

Alteration of the basement membrane in human thyroid diseases: An immunohistochemical study of type IV collagen,laminin and heparan sulphate proteoglycan

Basement membrane (BM) alteration in thyroid diseases was examined by immunohistochemistry using antibodies for the three major BM proteins: type IV collagen, laminin and heparan sulphate proteoglycan. Linear epithelial BMs surrounding follicles accompanied by vascular BMs forming loops, similar to those seen in the normal thyroid, were observed in Graves' disease and adenomatous goitre. Hashimoto's thyroiditis showed scant epithelial BMs as a result of follicle destruction. In follicular adenomas, development of epithelial BMs seemed to be related to follicle formation; well-developed epithelial BMs were frequently seen in normo- or largefollicular type, whereas trabecular or solid types revealed scant or poorly developed epithelial BMs. Lumpy accumulation of BM proteins was detected in hyalinizing trabecular adenomas. Papillary carcinomas revealed two different types of papillae; one type contained both epithelial and vascular BMs, and the other had only vascular BMs. Epithelial BMs in invasive areas of papillary carcinoma were distributed in an irregular, interrupted manner, and were completely absent in many foci. Anaplastic carcinomas showed scant or a total loss of epithelial BMs. These results suggest that alterations of BM in thyroid diseases clearly reflect their architectural variations, presumably in connection with their function and/or biological behaviour.     

Immunohistochemical localization of macromolecules of the basement membrane and the peritumoral stroma in human laryngeal carcinomas

Forty laryngeal carcinomas were studied by immunofluorescence with specific antisera against components of the basement membrane (type IV collagen and laminin) as well as antisera against connective tissue antigens (type V collagen and fibronectin). The basement membrane surrounding well-differentiated squamous cell carcinomas showed an appearance similar to that seen beneath normal epithelium. In contrast, marked alterations of the basement membrane were constantly observed around infiltrating and poorly-differentiated carcinomas. The staining of connective tissue components in most cases was as intense in carcinomas as in normal laryngeal mucosa. The use of antibodies to basement membrane components may help to elucidate the mechanism of invasion of connective tissues by malignant cells.     

Basement membrane proteins and reticulin in a normal thymus and the thymus in myasthenia gravis

Summary The distribution of basement membrane (BM) proteins, laminin and type IV collagen were studied immunohistochemically in a series of 12 normal thymuses representing different age groups (0–52 years) and in 10 cases of myasthenia gravis (age 7–53 years). The staining pattern was compared with that of conventional reticulin staining. BM proteins were present at the capsule-parenchyma interface and scantily distributed in the medullary stroma, where they were closely associated with reticulin fibres. The extrathymic perivascular space was effectively vizualized by the staining of the BM's marginal to it. The fiber network present in this space stained with reticulin stain and, less continuously, in BM stainings. Lymph node like tissue with germinal centers was occasionally present in the perivascular spaces in normal thymuses and commonly in the myasthenia gravis cases, where the perivascular spaces were often dilated. The BM's of the perivascular space were mostly continuous in normal cases, but discontinuities were observed in cases of myasthenia gravis, especially in the spaces which were widely dilated. Immunohistochemical detection of BM proteins seems to be useful in the study of thymic structure, particularly in the demonstration of the characteristic changes of the perivascular space in myasthenia gravis. It is suggested that the reticulin fibres present in the medulla and in the perivascular space contain laminin and type IV collagen.     

人绒毛膜促性腺激素单克隆抗体的研制

目的获得针对人绒毛膜促性腺激素单克隆抗体。方法hCG蛋白免疫Balb／c小鼠,取其脾细胞与同系小鼠骨髓瘤细胞NS-1按8：1比例融合,间接ELISA法筛选阳性克隆,有限稀释法进行克隆化培养;制备腹水抗体;采用间接ELISA法鉴定抗体亚型和测定抗体效价。结果得到6株能稳定分泌单克隆抗体的杂交瘤细胞株;抗体经鉴定均为IgG1、κ型,效价均达10^-5以上。结论所获得的6株杂交瘤细胞株均有较强稳定分泌抗-hCG单克隆抗体的能力。这为有关hCG的检测、hCG本身相关研究以及避孕疫苗的研制打下了基础。     

Production and characterization of monoclonal antibodies against non-A1c glycated hemoglobin

Hybridomas secreting monoclonal antibodies specific for hemoglobin nonenzymatically glycated in the non-A_1c position were produced by fusion of SP 2/0 myeloma cells with spleen cells from BALB/c mice immunized with nonenzymatically glycated hemoglobin prepared from human erythrocytes. Wells containing hydridomas secreting antibodies against glycohemoglobin were identified by binding, in an enzyme-linked immunosorbent assay, to purified glycated hemoglobin. The colony designated E85, which secreted antibodies discriminating between glycated versus unglycated hemoglobin, was cloned at least four times by limiting dilution and used for further study, performed with purified monoclonal antibody. Specificity of E85 was demonstrated by immunoblotting and by ELISA, wherein the monoclonal antibody reacted with glycated hemoglobin but not with hemoglobin A_1c or with unglycated hemoglobin. Immunoblotting of human plasma with E85 on nitrocellulose yielded no reactive proteins, indicating site specificity for glycated epitopes residing in hemoglobin but not in other nonenzymatically glycated proteins present in plasma. E85 differs from other antibodies raised against glycated hemoglobin and other glycated proteins, which recognize hemoglobin glycated at the N terminal valine of the β chain (HbA_1c) or which recognize glycated residues only after reductive conversion to glucitollysine and which do not discriminate between different glycated proteins. Thus, this report describes the establishment of the first hybridoma secreting monoclonal antibody raised against a physiologic (unreduced) form of non-A_1c glycohemoglobin, and for the glycated epitope when it resides in glycohemoglobin but not in other proteins or in hemoglobin A_1c.     

p38MAPK参与高糖刺激大鼠肾小管上皮细胞产生细胞外基质胶原Ⅲ

目的：探讨p38MAPK信号通路在高糖刺激大鼠肾小管上皮细胞产生细胞外基质胶原Ⅲ中的作用。 方法： 采用体外培养和Western blotting等方法，以不同浓度D-葡萄糖、p38MAPK信号通路特异性阻断剂SB203580以及用不同时间刺激正常大鼠肾小管上皮细胞NRK52E，分别检NRK52E细胞p38MAPK磷酸化水平和细胞外基质胶原Ⅲ的表达。 结果： 随D-葡萄糖浓度增加，p38MAPK磷酸化水平、胶原Ⅲ的产生也增加，SB203580可有效阻断高糖引起p38MAPK磷酸化水平的升高和细胞外基质胶原Ⅲ的表达的增高。 结论： 高糖引起p38MAPK磷酸化水平的升高可能在糖尿病肾病的肾间质纤维化中发挥重要作用。SB203580有潜在的糖尿病肾病防治的临床应用价值。     

The immunocytochemical demonstration of basement membrane deposition in transitional cell carcinoma of bladder

Summary We assessed the staining characteristics of the basement membrane of transitional cell carcinoma of bladder using a monoclonal antibody to type IV collagen. Basement membranes were clearly stained at the stromal/carcinoma interface. As transitional cell carcinoma became less well differentiated and the depth of invasion increased interruptions to basement membrane staining became more extensive and these findings are comparable to those described in similar series of transitional cell carcinoma using polyclonal antibodies to type IV collagen. The defects in basement membrane staining may be related to the degree and direction of tumour cell differentiation or may be explained by increased degradation compared to synthesis of basement membrane components. Demonstration of the basement membrane may be of value in diagnostic histopathology as a marker of the biological behaviour of transitional cell carcinoma of bladder.     

人胱抑素C单克隆抗体的制备、鉴定及初步应用

目的:制备人胱抑素C(Cystatin C,Cys C)的单克隆抗体(McAb),并建立检测人血清Cys C的颗粒增强透射免疫浊度分析法(PETLA).方法:构建人Cys C的原核表达载体pET32a( )/Cys C,纯化Cys C重组蛋白并免疫BALB/c小鼠,杂交瘤技术制备Cys C的McAb;以自制的McAb包被乳胶颗粒,建立PETIA法测定血清Cys C,并对其分析性能进行初步方法学评价.结果:建立分泌抗Cys C单克隆抗体的杂交瘤细胞株3株,其分泌的McAb为IgG1,Western blot检测证实该抗体能与目的蛋白发生特异性结合;将杂交瘤细胞注射于小鼠腹腔,腹水中Cys C McAb效价为1∶4×106;用自制的McAb建立定量测定Cys C的PETIA,方法学评价试验结果证实我们建立的PETIA法,与进口试剂有很好的可比性,具有较满意的方法学性能.结论:成功制备了抗Cys C单克隆抗体,该抗体可用于建立定量检测Cys C的PETIA法.     

抗人粒细胞单克隆抗体的特异性鉴定及其核素99Tcm标记

目的以人粒细胞免疫Balb/c小鼠制备抗粒细胞单克隆抗体(mAb),并对其组织特异性进行鉴定,同时评价其在兔炎症模型中的显像价值。方法常规免疫制备抗粒细胞mAb经间接ELISA法、流式细胞仪和SP免疫组化进行特异性鉴定。99Tcm间接法标记SZ102。兔左下肢炎症模型制备完毕,耳缘静脉注入99TcmSZ1024h后探讨其在兔炎症模型中的体内分布。结果制备抗粒细胞mAbSZ102,其免疫球蛋白亚类为IgG1。流式细胞仪测定表明其与外周血粒细胞、单核细胞呈强阳性反应,而与淋巴、红细胞、血小板不反应,并且与正常骨髓中较成熟粒细胞、单核前体起反应。SP免疫组化法检测正常人组织中SZ102抗原分布,显示抗原表达在肝、肺、脾、胸腺、淋巴结组织中的巨噬细胞表面。注射99TcmSZ1024h后,离体炎症肌肉/血液和对侧正常肌肉/血液单位质量放射性比值分别为0.22±0.02和0.02±0.01。结论SZ102是一株稳定高效价抗粒细胞杂交瘤细胞株,99TcmSZ102具有活体内炎症定位导向能力,对隐匿性炎症的放免显像可能有一定的诊断价值。     

Immunohistochemical methods for semiquantitative analysis of collagen content in human peripheral nerve

Methods are described for the semiquantitative analysis of the connective tissue components of human peripheral nerve using light microscopy. General histological preservation was assessed using haematoxylin and eosin staining and the distribution of collagen type IV was investigated using immunohistochemistry. Several techniques were investigated to establish the one giving optimum structural preservation, immunobinding and greatest contrast for image analysis. Frozen sections were unsuitable for this tissue and paraffin wax sections were therefore used. Alcohol fixation was rejected due to poor preservation of the endoneurium, although immunobinding was excellent. Ice-cold formalin fixation for 24 h was found to be adequate for structural preservation and antibody binding, provided that a protease step was introduced. Trypsin was found to be superior to pepsin for exposing collagen type IV epitopes. Of the detection systems investigated indirect immunofluorescence was not suitable due to considerable autofluorescence of the nerve. The avidin-biotin method provided the greatest contrast, and was therefore the detection method of choice for image analysis. The optimum techniques for image analysis were then used on control human sural nerve to ascertain the best comparative method for collagen type IV in the perineurium. A method of semiquantitative analysis is described which takes into account the fact that there is a close linear relationship between collagen content per unit of perineurium and perineurial perimeter as fascicle size increases in peripheral nerve. This means that data from 2 different sample groups can easily be compared, provided that a range of fascicle sizes is analysed in each case.