Progress of Domestic Recombinant Human-Like Collagen Research and Application

By intercepting the most effective fragment of human collagen’s gene,recombinant human-like collagen is produced by genetic engineering technology and biotechnology.The collagen has good biocompatibility and can promote cell formation.Recombinant human-like collagen has great potential application value in medical biological materials,cosmetics and foods.In recent years,many specialized enterprises which are engaged in human-like collagen raw materials production have emerged.In this paper,a brief summary of the current recombinant human-like collagen raw material’s production and its latest research and development have been made.

Mineralization of Hydroxyapatite Regulated by Recombinant Human-like Collagen

We reported recombinant human-like type I collagen inducing growth of hydroxyapatite crystals in vitro in the form of self-assembly of nano-fibrils of mineralized collagen resembling extracellular matrix, which obey the same rules, but is superior to the collagen derived from animal tissues because the latter may carry diseases of animals and cause immunological reactions. The mineralized collagen fibrils aligned parallel to each other to form mineralized collagen fibers. Hydroxyapatite nanocrystals grew on the surface of these collagen fibrils with the c-axis of nanocrystals of HA orienting along the longitudinal axis of the fibrils.

Skin care efficacy study of recombinant humanized collagen based on in vitro level

Studying the skin care efficacy of recombinant humanized collagen based on in vitro level.The stability of the recombinant humanized collagen was first analyzed by treating at different temperatures,then its skincare efficacy based on in vitro level was evaluated by detecting the inhibition rate of elastase,the inhibition rate of collagenase,the protein content of type I collagen in human fibroblasts,the inhibition of reactive oxygen species(ROS)with human keratinocytes,and the effects of the recombinant humanized collagen on the expression of hyaluronic acid(HA),filaggrin(FLG)and transglutaminase 1(TGM1)in keratinocytes.The results showed that recombinant humanized collagen was able to maintain stability at temperatures below 70℃.With regard to its skincare efficacy,recombinant humanized collagen could inhibit elastase and collagenase activities and promote the increase of type I collagen content in human fibroblasts.It also showed good inhibition of ROS in keratinocytes in vitro and could increase the expression of HA,FLG,and TGM1 in keratinocytes.In short,the recombinant humanized collagen exhibited a favourable skin care effect in vitro level.This study proved that it has potential firming,anti-wrinkle,moisturizing,and repairing efficacy,and is a valuable cosmetic raw material.

Optimization of Fermentation Process for Human-like Collagen Production of Recombinant Escherichia coli Using Response Surface Methodology

In order to improve the production of human-like collagen III(HLC III)by fed-batch culture of recombinant Escherichia coli BL21,the Plackett-Burman and Box-Behnken design were applied to optimize the fermentation process parameters.Three variables(induction time,inoculum age and pH),which have significant effects on HLC III production,were selected from eight variables by Plackett-Burman design.With the regression coefficient analysis in the Box-Behnken design,a relationship between HLC III production and three significant factors was obtained,and the optimum levels of the three variables were as follows:induction time 3.2h,inoculum age 12.6 h and pH 6.7.The 3D response surface plots and 2D contour plots created by the Box-Behnken design showed that the interaction between induction time and pH and that between innoculum age and pH were significant.An average 9.68 g·L1HLC III production was attained in the validation experiment under optimized condition,which was 80%higher than the yield of 5.36 g·L1before optimization.

Kinetics of High Cell Density Fed-batch Culture of Recombinant Escherichia coli Producing Human-like Collagen

The kinetics of batch and fed-batch cultures of recombinant Escherichia coli producing human-like collagen was investigated. In the batch culture, a kinetic model of a simple growth-association system was concluded without consideration of cell endogeneous metabolism. The cell lag time, the maximum specific growth rate and Yx/s were determined as 1.75h, 0.65h^-1 and 0.51g·g^-1, respectively. In the fed-batch culture, different specific growth rates were set at （0.15, 0.2, 0.25h^-1） by the method of pseudo-exponential feeding, and the expressions for the specific rate of substrate consumption, the growth kinetics and the product formation kinetics of each phase were obtained. The result shows that the concentrations of cell and product can reach 77.5g·L^-1 and 10.2g·L^-1 respectively. The modal predictions are in good agreement with the experimental data.

Analysis of Metabolic Products by Response Surface Methodology for Production of Human-like Collagen II

Recombinant Escherichia coli BL21 is used to produce human-like collagen. The key constituents of media are optimized using response surface methodology (RSM). Before thermal induction, the highest biomass production and the lowest production of some hazardous by-products, especially acetic acid, were obtained in the media containing 0.085 mol·L-1 glucose and 0.019 mol·L-1 nitrogen (carbon-nitrogen ratio, 4.47:1). After thermal induction, when the concentrations of glucose and nitrogen in the media were 0.065 mol·L-1 and 0.017 mol·L-1 , respectively (carbon-nitrogen ratio, 3.82:1), the productivity of human-like collagen per cell was the highest while that of acetic acid was the lowest. The extended analysis showed that the production of lactic acid and propionic acid increased while that of some intermediate acids of the tricarboxylic acid cycle decreased if the dose of glucose increased.

Process Control for Production of Human-like Collagen in Fed-batch Culture of Escherichia coli BL 21

Recombinant E. coli BL 21 was cultivated in high cell density to produce human-like collagen. The effects of the feeding of nitrogen source, controlled by an auto on/off-feeding mode with two different cycles of 0.5min and 4min intervals, oxygen-enrichment methods and inducement strength on the cell yield and human-like collagen production were investigated. The studies showed that nitrogen source feeding in fast cycle could result in higher human-like collagen production than that in slow cycle; and the feedback regulation of glucose, increase of the pressure of fermentation bioreactor, and supply of oxygen-enriched air could all increase cell yield and human-like collagen production. The effects of inducement strength on protein expression were found important. When OD600 reached 90-100, the cultivation temperature was increased to 42℃ to begin induction for 2-3 h, and then shifted to 39℃ for 5-6h induction, the cell density and human-like collagen production could reach 96g·L-1 [DCW (dry cell mass)] and 19.8% (g·g-1 DCW) respectively.

Status and developmental trends in recombinant collagen preparation technology

Recombinant collagen is a pivotal topic in foundational biological research and epitomizes the application of critical bioengineer-ing technologies.These technological advancements have pro-found implications across diverse areas such as regenerative medicine,organ replacement,tissue engineering,cosmetics and more.Thus,recombinant collagen and its preparation methodologies rooted in genetically engineered celis mark pivotal milestones in medical product research.This article pro-vides a comprehensive overview of the current genetic engi-neering technologies and methods used in the production of recombinant collagen,as well as the conventional production process and gquality control detection methods for this material.Furthermore,the discussion extends to foresee the strides in physical transfection and magnetic control sorting studies,envisioning an enhanced preparation of recombinant collagen-seeded cells to further fuel recombinant collagen production.

Versatile dopamine-functionalized hyaluronic acid-recombinant human collagen hydrogel promoting diabetic wound healing via inflammation control and vascularization tissue regeneration

The management of chronic wounds in diabetes remains challenging due to the complexity of impaired wound healing,delayed healing,susceptibility to infection,and elevated risk of reopening,highlighting the need for effective chronic wound management with innovative approaches such as multifunctional hydrogels.Here,we have produced HA-DA@rhCol hydrogels consisting of dopamine-modified hyaluronic acid and recombinant human collagen type-III(rhCol)by oxidative coupling of the catechol group using the H_(2)O_(2)/HRP catalytic system.The post-reactive hydrogel has a good porous structure,swelling rate,reasonable degradation,rheological and mechanical properties,and the catechol group and dopamine impart to the hydrogel tissue adhesiveness,antioxidant capacity,and excellent photothermal effects leading to superior in vitro antimicrobial activity.In addition,the ability of rhCol to confer hydrogels to promote angiogenesis and wound repair has also been investigated.Cytotoxicity and hemolysis tests demonstrated the good biocompatibility of the hydrogel.Wound closure,collagen deposition and immunohistochemical examination confirmed the ability of the hydrogel to promote diabetic wound healing.In summary,the adhesive hemostatic antioxidative hydrogel with rhCol to promote wound healing in diabetic rat is an excellent chronic wound dressing.

Active Peptides and Motifs within Collagen and Other ECM Proteins

Collagens are the most abundant proteins in mammals and form an extracellular matrix (ECM) with other components as the structural support of muscle, skin, corneas and blood vessels etc. Other than providing structural support, the ECM exhibits active communication with cells and influences many cellular processes including migration, wound healing, differentiation and cancer metastasis. Though collagen proteins contain highly repetitive primary sequences and defined tertiary structures, more and more studies have shown that many short peptides/motifs within collagen proteins play key roles in various biological processes. These short sequences are effective within triple helical structures or independently as stand-alone molecules resulting from proteolytic degradation. Besides endogenous ECM-derived peptides, many more functional peptides have been produced by tissue processing, chemical synthesis, and recombinant protein production. In this review, we summarize different peptides/motifs identified in collagen and other ECM proteins and discuss their potential for medical, personal care, and cosmetics applications.

微针导入重组Ⅲ型人源化胶原蛋白在皮肤屏障功能修复中的应用效果

目的探究微针导入重组Ⅲ型人源化胶原蛋白治疗因皮肤炎性衰老导致的皮肤屏障功能下降的有效性及安全性。方法选取2020年6月至2021年5月在本院接受面部皮肤治疗的30例患者作为研究对象,采用随机数字表法将其分为对照组(重组Ⅲ型人源化胶原蛋白)与治疗组(微针导入重组Ⅲ型人源化胶原蛋白),各15例。治疗后定期对患者进行随访,分别进行主观疗效评价及客观疗效评价。结果治疗后4、8、12周,治疗组的满意度显著高于对照组(P<0.05)。治疗后,治疗组的皮肤皱纹、纹理、红区、毛孔、弹性、皮肤经皮失水及皮肤含水量改善明显(P<0.05);对照组治疗后油脂改善明显(P<0.05)。治疗后12周,治疗组的总症状评分显著低于对照组(P<0.05)。结论微针导入重组Ⅲ型人源化胶原蛋白对皮肤修复有较好的疗效,可增强皮肤屏障功能,为改善皮肤屏障功能、治疗因皮肤屏障受损引起的炎性衰老提供了新选择。

补充重组人源胶原蛋白对离心运动后小鼠骨骼肌细胞外基质重塑的影响

背景:胶原蛋白是含量最为丰富的胞外基质成分,与骨骼肌细胞外基质的结构、功能密切相关,但补充由生物工程技术生产的重组人源胶原蛋白(recombinant human collagen,rhC)对骨骼肌细胞外基质的影响及机制尚不清楚。目的:探讨补充rhC对离心运动后骨骼肌细胞外基质重塑的影响及作用机制。方法:将104只8周龄健康雄性C57小鼠随机分为对照组(生理盐水)、rhC低剂量组(0.2 g/kg)、中剂量组(1.0 g/kg)和高剂量组(2.0 g/kg),连续7 d灌胃干预后每组选取2只小鼠,解剖各脏器进行苏木精-伊红染色判断炎性浸润情况,其余小鼠于第8天进行离心运动,分别在离心运动后即刻(0),24,48,96 h观察细胞外基质结构变化,检测小鼠抓握力、血清肌酸激酶活性、骨骼肌组织基质金属蛋白酶2,9,14和基质金属蛋白酶抑制剂2的蛋白水平。结果与结论:①苏木精-伊红染色观察短期补充rhC对心脏、肝脏、脾、肾无显著影响;②一次性离心运动后,rhC中、高剂量组小鼠抓握力恢复率显著升高(P<0.01);③各组肌酸激酶变化趋势一致,组间无显著性差异;④rhC低剂量组细胞外基质恢复进程快于对照组,rhC中、高剂量组肌束膜较为完整;⑤rhC高剂量组基质金属蛋白酶9蛋白水平显著降低(P<0.05);⑥rhC中、高剂量组基质金属蛋白酶14蛋白水平显著降低(P<0.05);⑦rhC中、高剂量组基质金属蛋白酶2蛋白水平显著降低(P<0.05);⑧rhC中、高剂量组基质金属蛋白酶抑制剂2蛋白水平显著升高(P<0.05);⑨rhC各剂量组基质金属蛋白酶2/基质金属蛋白酶抑制剂2比值显著降低(P<0.05)。该研究发现连续7 d预补充1.0,2.0 g/kg rhC可通过调节基质金属蛋白酶和基质金属蛋白酶抑制剂来抑制运动后骨骼肌细胞外基质降解,从而促进小鼠骨骼肌力量恢复。

携载重组胶原蛋白的卡波姆凝胶喷剂制备及对大鼠口腔溃疡愈合作用观察

目的 制备携载重组胶原蛋白的卡波姆凝胶喷剂,并观察其对大鼠口腔溃疡的愈合作用。方法 选取可用于口服制剂的卡波姆971P为主要材料,添加不同质量浓度的甘油、磷酸二氢钾(KH2PO4)、Ⅲ型重组胶原蛋白(rhColⅢ)等制备凝胶喷剂,观察凝胶喷剂在不同pH下的喷出性能、不同缓冲剂对凝胶喷剂粘度变化的影响、不同pH卡波姆凝胶对胶原蛋白溶解度的影响。使用醋酸灼烧法建立大鼠口腔溃疡模型,模型建立成功后随机分为空白对照组、卡波姆组(采用不含胶原蛋白的卡波姆凝胶喷剂治疗)、胶原蛋白组(采用含rhColⅢ的卡波姆凝胶喷剂治疗),比较各组大鼠溃疡愈合率及黏膜组织HE染色结果。结果 卡波姆粘度在2 500~3 000 mpa·s时具有良好的喷出性能。随着离子溶度的升高,卡波姆粘度不断下降(P均<0.05)。当凝胶pH是4时,卡波姆中有大量白色团块(未溶解的胶原蛋白),继续延长搅拌时间白色团块未减少;往凝胶中继续缓慢少量添加KOH并不断搅拌,随着pH不断升高,白色团块不断减小,当pH升高到5左右,白色团块消失。空白对照组、卡波姆组、胶原蛋白组制模后第3天溃疡愈合率分别为38.7%、45.6%、53.1%,空白对照组与胶原蛋白组相比,P<0.05;空白对照组、卡波姆组、胶原蛋白组制模后第5天溃疡愈合率分别为62.9%、72.4%、88.5%,胶原蛋白组分别与空白对照组、卡波姆组比较,P均<0.05。制模后第3天,各组口腔黏膜上皮处均有缺损,空白对照组缺损最大,上皮层和固有层中单核细胞、多形核细胞等炎症细胞数量较多,新生血管数量较少;相比于空白对照组,卡波姆组炎症细胞数量减少,新生血管数量较多;而相比于其他两组,胶原蛋白组炎症细胞相对最少,新生血管数量较多,且缺损面积减少;制模后第5天,空白对照组黏膜上皮尚有缺损,炎症细胞数量较多;相比于空白对照组,卡波姆组上皮缺损和炎症细胞数量减少,新生血管数量较多;阳性对照组相比于其他两组,炎症细胞数量最少,新生血管数量明显增多,上皮缺损已完全愈合。结论 携载重组胶原蛋白的卡波姆喷剂具有良好的喷出性能和粘附性能,该喷剂能显著促进大鼠口腔溃疡的愈合。

玻璃体内注射原纤维蛋白-2(FBN2)重组蛋白对FBN2缺陷型视网膜病变的影响

目的探讨玻璃体内注射原纤维蛋白-2(FBN2)重组蛋白对FBN2缺陷型视网膜病变的影响。方法取SPF级C57BL/6J小鼠32只,随机分为4组:正常对照组、阴性对照组、FBN2敲减组、FBN2重组蛋白组,每组8只小鼠,取右眼作为实验眼。入组后,正常对照组小鼠不进行干预,阴性对照组小鼠玻璃体内注射3μL空载体(1 mg·L^(-1)),FBN2敲减组及FBN2重组蛋白组小鼠玻璃体内注射3μL腺相关病毒(AAV)(1 mg·L^(-1)),4周后FBN2重组蛋白组小鼠玻璃体内注射3μL FBN2重组蛋白(1 mg·L^(-1))。采用视网膜电图(ERG)视觉电生理仪和光学相干断层扫描(OCT)仪分别检测小鼠视网膜Rod-b、Max-a波振幅和视网膜结构变化;RT-PCR、Western blot检测小鼠视网膜中FBN2、微原纤维相关糖蛋白(MAGP-2)、Ⅰ型胶原蛋白(COL1)mRNA和蛋白表达变化。结果ERG检测结果显示,与阴性对照组和正常对照组相比,FBN2敲减组和FBN2重组蛋白组小鼠视网膜ERG Rod-b、Max-a波振幅均变小(均为P<0.05);与FBN2敲减组相比,FBN2重组蛋白组视网膜ERG Rod-b、Max-a波振幅均明显增加(均为P<0.05)。OCT检测结果显示,与FBN2敲减组相比,FBN2重组蛋白组小鼠视网膜色素上皮层组织结构恢复正常,光反射变规则。RT-PCR检测结果显示,与FBN2敲减组相比,FBN2重组蛋白组小鼠视网膜组织FBN2 mRNA表达明显升高,COL1、MAGP-2 mRNA表达均明显降低(均为P<0.05)。Western blot检测结果显示,与FBN2敲减组相比,FBN2重组蛋白组小鼠视网膜组织FBN2蛋白表达明显升高,COL1、MAGP-2蛋白表达均明显降低(均为P<0.05)。结论玻璃体内注射FBN2重组蛋白可以弥补FBN2缺陷型视网膜病变小鼠FBN2内源性缺失,通过调控COL1、MAGP-2表达可达到治疗疾病的作用。

EDC/NHS交联重组胶原蛋白水凝胶修复关节软骨缺损

关节软骨损伤、缺损是一种常见且严峻的临床挑战,没有有效的治疗方法,基于胶原蛋白的水凝胶是软骨组织工程的研究热点之一,但在开发具有良好生物相容性且可安全交联的胶原蛋白产品,并提高软骨修复有效性方面仍然存在巨大挑战。将重组Ⅰ型胶原蛋白和重组Ⅲ型胶原蛋白通过EDC/NHS交联,制备了2种水凝胶,均表现出良好的三维孔隙结构以及优异的力学性能和可降解性。研究发现,重组Ⅰ型胶原蛋白水凝胶(Gel-Ⅰ)和重组Ⅲ型胶原蛋白水凝胶(Gel-Ⅲ)能促进人骨髓间充质干细胞(human bone-marrow mesenchymal stem cells,HBMSCs)糖胺聚糖的分泌,Gel-Ⅰ可以显著上调HBMSCs表达COLⅡ基因和SOX9基因,Gel-Ⅲ可以显著上调SOX9基因表达。在兔子膝关节软骨修复模型中,与对照组和Gel-Ⅲ组相比,Gel-Ⅰ组在骨体积大小方面表现出明显优势,软骨下骨已形成并有效恢复,小梁的数量和厚度最高,小梁分布更均匀,并且缺损处新软骨厚度与相邻软骨厚度相同。因此,Gel-Ⅰ在软骨修复有效性以及安全性方面具有极大的临床应用潜力。

表达元件优化促进重组胶原蛋白在谷氨酸棒杆菌中的表达

重组胶原蛋白是一种具有广泛应用潜力的生物材料,近年来引起了生物医学、组织工程等众多领域的关注。胶原蛋白的3股螺旋结构赋予其独特的生物学功能和生物相容性,但也增加了其在微生物系统中表达的复杂性。该研究以细菌胶原蛋白V-B作为模式蛋白,通过对表达元件的优化,促进重组胶原蛋白在谷氨酸棒杆菌中的表达。首先通过启动子筛选和发酵时长优化,获得介导V-B表达的最优启动子tac-R0。接着利用RBS calculator设计核糖体结合位点(ribosomal binding site,RBS)和间隔序列(aligned spacing,AS)的突变文库,得到与tac-R0启动子搭配组合的最优RBS和AS,使V-B的产量提高至514 mg/L。此外,通过多基因表达盒的串联组合策略,将多个目的基因串联,最终V-B的产量较初始水平提高了8.4倍,达697 mg/L,该研究为重组胶原蛋白的工业化生产提供了基础。

强脉冲光联合酵母重组胶原蛋白凝胶治疗面部糖皮质激素依赖性皮炎疗效观察

目的:探讨强脉冲光(Intense pulsed light,LPL)联合酵母重组胶原蛋白凝胶治疗面部糖皮质激素依赖性皮炎(Facial hormone dependent dermatitis,FHDD)的效果。方法:将2021年1月-2022年3月笔者医院收治的100例FHDD患者随机均分为观察组和对照组,每组50例。两组均采用IPL及其他常规措施治疗,观察组加涂酵母重组胶原蛋白凝胶治疗,对照组加涂安慰剂(酵母重组胶原蛋白模拟状凝胶)。比较治疗前后两组疗效、皮肤生理参数、血清炎症因子和免疫球蛋白水平、皮肤病生活质量指数(Dermatology life quality index,DLQI)。结果:观察组治疗总有效率80.00%高于对照组52.00%(P<0.05)。治疗后,两组经皮水分散失(Transepidermal water loss,TEWL)水平、血清白细胞介素(IL-4)、干扰素(IFN-γ)、免疫球蛋白(IgE、IgA、IgM)水平、DLQI量表评分均较治疗前降低,且观察组低于对照组(P<0.05)。两组患者表皮皮脂含量和角质层含水量较治疗前升高,且观察组高于对照组(P<0.05)。两组患者不良反应发生率比较差异无统计学意义(P>0.05)。随访6个月,观察组复发率5.00%低于对照组25.00%(P<0.05)。结论:IPL联合酵母重组胶原蛋白凝胶治疗FHDD效果确切,能改善皮肤生理参数,调节血清炎症因子和免疫球蛋白水平,提高患者生活质量。

医用重组人源胶原蛋白功能敷料体外免疫原性评价

目的对一种医用重组人源胶原蛋白功能敷料的体外免疫原性进行评价。方法以细胞培养液为浸提介质,按0.2 g/ml的比例浸提制备试验液,进行体外淋巴细胞增殖试验、人细胞系激活试验(h-CLAT)、细胞炎症因子含量检测。结果体外淋巴细胞增殖试验中,100%,50%,25%3种浓度试验液的淋巴细胞增殖率分别为105%,111%,86.3%,与阴性对照组比较,差异无统计学意义(P>0.05)。h-CLAT结果显示,试验组THP-1细胞表面分子CD54 RFI值<200,CD86 RFI值<150,判定为阴性结果。试验组细胞上清中肿瘤坏死因子α(TNF-α)、白介素8(IL-8)的含量与阴性对照组比较,差异无统计学意义(P>0.05)。结论医用重组人源胶原蛋白功能敷料有良好的生物相容性。

Recombinant humanized collagen remodels endometrial immune microenvironment of chronic endometritis through macrophage immunomodulation

Recently,evidence has suggested that chronic endometritis(CE)is a crucial factor associated with infertility and failure of assisted reproductive techniques,prompting concern in the reproductive field.Studies have shown that persistent infiltered immune cells stimulation result in the disturbance of endometrial immune microenvironment could lead to the infertility of CE patients finally.Conventional treatments are limited because they lack immune regulation,so it is urgent to develop a novel approach to treat CE and promote embryo implantation in patients with CE.Herein,we prepared recombinant humanized type III collagen(rhCol III)with high cell adhesion activity to regulate macrophages and repair the endometrium.In this study,M1 macrophages and M1 macrophages cultured medium and lipopolysaccharide(LPS)co-stimulated inflammatory endometrium stromal cells(ESCs)were established in vitro to mimic CE condition.rhCol III promoted M1 macrophages toward M2 phenotype,improved cell migration,viability and collagen components of inflammatory ESCs.Also,the inflammatory response of inflammatory ESCs was downregulated after rhCol III treatment.Subsequently,LPS was used for CE rat model and a 28-day observation was performed;inflammatory cells’infiltration,endometrium repair,extracellular matrix(ECM)remodeling and pregnancy outcomes were promoted after rhCol III endometrial infusion.In conclusion,rhCol III promoted(i)macrophage polarization toward M2 macrophages,(ii)pro-inflammatory cytokine production and anti-inflammatory cytokine reduction,(iii)ECM remodeling and(iv)fertility restoration.Meanwhile,rhCol III enhanced cell biological functions by interacting with discoidin domain receptors,regulated cell metabolism and reduced the inflammatory response through the inhibition of the NF-κB/YAP signaling pathway.Overall,the results illustrated the potential therapeutic prospects of rhCol III for CE treatment.

胶原酶治疗胶原蛋白(刺激剂)植入后结节并发症专家共识

1概述。2胶原蛋白(刺激剂)及其植入后结节并发症。2.1胶原蛋白。2.2胶原蛋白及胶原蛋白刺激剂在医疗美容中的应用。2.2.1胶原蛋白(刺激剂)植入适应证。2.2.2胶原蛋白(刺激剂)植入后常见的并发症。2.3胶原蛋白(刺激剂)植入后结节并发症。2.4胶原蛋白(刺激剂)植入后结节并发症的治疗。3胶原酶在胶原蛋白(刺激剂)植入术后结节并发症治疗中的应用。3.1胶原酶及其在临床中的应用。3.2胶原酶治疗胶原蛋白(刺激剂)植入术后结节并发症的理论基础及实验结果。3.3局部注射胶原酶治疗胶原蛋白(刺激剂)植入术后结节的操作方法。3.3.1适应证。3.3.2禁忌证。3.3.3注射方法。3.3.4操作注意事项。3.3.5治疗后护理。3.4局部注射胶原酶的不良反应及处理措施。4总结。