组织工程与重建外科杂志
組織工程與重建外科雜誌
조직공정여중건외과잡지
JOURNAL OF TISSUE ENGINEERING AND RECONSTRUCTIVE SURGERY
2013年
6期
311-314
,共4页
生物膜%自体颅骨粉末%颅骨缺损%移植%修复%组织学演变
生物膜%自體顱骨粉末%顱骨缺損%移植%脩複%組織學縯變
생물막%자체로골분말%로골결손%이식%수복%조직학연변
Membrane%Autogenous skull bone dust%Cranial defects%Transplantation%Repairment%Histological evolution
目的:应用自体颅骨粉末移植和膜引导再生技术修复兔颅骨缺损模型,观察其组织学演变过程。方法选取50只新西兰大白兔,建立直径1 cm的颅骨全层缺损模型。移植自体骨粉修复兔颅骨缺损,并在移植的骨粉上放置可吸收生物膜,以纤维蛋白胶固定。术后2、4、6、8、12周取材进行组织学观察。结果术后2周,可观察到颅骨缺损区大量骨粉,炎性细胞、毛细血管和成纤维细胞由周围向内浸润,骨粉被吞噬吸收,周边小部分是新生骨,两者之间界限明显。术后4周,观察到骨粉吸收和新骨形成活跃区域向缺损中央内移较多,新生编织骨有所增粗,编织骨之间连接更为紧密,观察到的组织和细胞成分与术后2周时无明显变化。术后6周,基本观察不到未被吸收的骨粉,新生的编织骨变粗,联系更紧密。术后8周,完全观察不到骨粉,缺损中央部已形成单层新生骨,周边部形成的编织骨较为粗大,与正常骨紧密连接,形成初级骨髓腔。术后12周,缺损中央部形成双层新生骨,可见新生骨的改建和较为成熟的骨髓腔,腔内容物形态和成分与正常骨无区别。结论应用自体颅骨粉末移植和膜引导再生技术可以修复颅骨缺损,其组织学演变过程实质是引导性和诱导性骨再生的过程。
目的:應用自體顱骨粉末移植和膜引導再生技術脩複兔顱骨缺損模型,觀察其組織學縯變過程。方法選取50隻新西蘭大白兔,建立直徑1 cm的顱骨全層缺損模型。移植自體骨粉脩複兔顱骨缺損,併在移植的骨粉上放置可吸收生物膜,以纖維蛋白膠固定。術後2、4、6、8、12週取材進行組織學觀察。結果術後2週,可觀察到顱骨缺損區大量骨粉,炎性細胞、毛細血管和成纖維細胞由週圍嚮內浸潤,骨粉被吞噬吸收,週邊小部分是新生骨,兩者之間界限明顯。術後4週,觀察到骨粉吸收和新骨形成活躍區域嚮缺損中央內移較多,新生編織骨有所增粗,編織骨之間連接更為緊密,觀察到的組織和細胞成分與術後2週時無明顯變化。術後6週,基本觀察不到未被吸收的骨粉,新生的編織骨變粗,聯繫更緊密。術後8週,完全觀察不到骨粉,缺損中央部已形成單層新生骨,週邊部形成的編織骨較為粗大,與正常骨緊密連接,形成初級骨髓腔。術後12週,缺損中央部形成雙層新生骨,可見新生骨的改建和較為成熟的骨髓腔,腔內容物形態和成分與正常骨無區彆。結論應用自體顱骨粉末移植和膜引導再生技術可以脩複顱骨缺損,其組織學縯變過程實質是引導性和誘導性骨再生的過程。
목적:응용자체로골분말이식화막인도재생기술수복토로골결손모형,관찰기조직학연변과정。방법선취50지신서란대백토,건립직경1 cm적로골전층결손모형。이식자체골분수복토로골결손,병재이식적골분상방치가흡수생물막,이섬유단백효고정。술후2、4、6、8、12주취재진행조직학관찰。결과술후2주,가관찰도로골결손구대량골분,염성세포、모세혈관화성섬유세포유주위향내침윤,골분피탄서흡수,주변소부분시신생골,량자지간계한명현。술후4주,관찰도골분흡수화신골형성활약구역향결손중앙내이교다,신생편직골유소증조,편직골지간련접경위긴밀,관찰도적조직화세포성분여술후2주시무명현변화。술후6주,기본관찰불도미피흡수적골분,신생적편직골변조,련계경긴밀。술후8주,완전관찰불도골분,결손중앙부이형성단층신생골,주변부형성적편직골교위조대,여정상골긴밀련접,형성초급골수강。술후12주,결손중앙부형성쌍층신생골,가견신생골적개건화교위성숙적골수강,강내용물형태화성분여정상골무구별。결론응용자체로골분말이식화막인도재생기술가이수복로골결손,기조직학연변과정실질시인도성화유도성골재생적과정。
Objective To repair the skull defects by using autogenous skull bone dust grafting and membrane guided regeneration technology, and to investigate its histological evolution. Methods Fifty New Zealand white rabbits were selected. A whole thick defect with the diameter of 1 cm was created in the parietal bone of every rabbit. The defect was grafted with autogenous skull bone dust and two pieces of absorbable membrane on two side. After 2, 4, 6, 8, 12 weeks, the defects were harvested for histological observation. Results Two weeks after operation, a large number of bone meal was observed in the defect area. Inward infiltration of inflammatory cells, capillaries and fibroblasts were observed. Bone meal was swallowed in the central area, new bone was formed in the surrounding area and a clear boundary was observed between the two area. Four weeks after operation, the boundary had moved a lot to the central area. New woven bone was thickened, the connection between the woven bone became more closely. Tissue and cell components had no obvious change compared with 2 weeks after operation. Six weeks after operation, bone meal was almost absorbed, the woven bone became thicker and the connection was more closely. Eight weeks after operation, no bone dust could be observed, a monolayer new bone was formed in the central area. The woven bone in the surrounding area was relatively thick and closely connected with normal bone. The primary bone marrow cavity was formed. Twelve weeks after operation, double new bone was observed in the central area. New bone remodeling and mature bone marrow cavity were also observed. The morphology and composition of bone marrow cavity had no difference compared with normal bone. Conclusion Histological evolution of autogenous bone dust grafting and membrane guided regeneration technology to repair skull defects is guided and induced bone regeneration.
