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表达骨形态发生蛋白-2的肌肉衍生细胞对小鼠临界尺寸骨缺损愈合的影响。

Effect of bone morphogenetic protein-2-expressing muscle-derived cells on healing of critical-sized bone defects in mice.

作者信息

Lee J Y, Musgrave D, Pelinkovic D, Fukushima K, Cummins J, Usas A, Robbins P, Fu F H, Huard J

机构信息

Children's Hospital of Pittsburgh, Pennsylvania 15261, USA.

出版信息

J Bone Joint Surg Am. 2001 Jul;83(7):1032-9. doi: 10.2106/00004623-200107000-00008.

Abstract

BACKGROUND

Cells that express bone morphogenetic protein-2 (BMP-2) can now be prepared by transduction with adenovirus containing BMP-2 cDNA. Skeletal muscle tissue contains cells that differentiate into osteoblasts on stimulation with BMP-2. The objectives of this study were to prepare BMP-2-expressing muscle-derived cells by transduction of these cells with an adenovirus containing BMP-2 cDNA and to determine whether the BMP-2-expressing muscle-derived cells would elicit the healing of critical-sized bone defects in mice.

METHODS

Primary cultures of muscle-derived cells from a normal male mouse were transduced with adenovirus encoding the recombinant human BMP-2 gene (adBMP-2). These cells (5 yen 10(5)) were implanted into a 5-mm-diameter critical-sized skull defect in female SCID (severe combined immunodeficiency strain) mice with use of a collagen sponge as a scaffold. Healing in the treatment and control groups was examined grossly and histologically at two and four weeks. Implanted cells were identified in vivo with use of the Y-chromosome-specific fluorescent in situ hybridization (FISH) technique, and their differentiation into osteogenic cells was demonstrated by osteocalcin immunohistochemistry.

RESULTS

Skull defects treated with muscle cells that had been genetically engineered to express BMP-2 had >85% closure within two weeks and 95% to 100% closure within four weeks. Control groups in which the defect was not treated (group 1), treated with collagen only (group 2), or treated with collagen and muscle cells without adBMP-2 (group 3) showed at most 30% to 40% closure of the defect by four weeks, and the majority of the skull defects in those groups showed no healing. Analysis of injected cells in group 4, with the Y-chromosome-specific FISH technique showed that the majority of the transplanted cells were located on the surfaces of the newly formed bone, but a small fraction (approximately 5%) was identified within the osteocyte lacunae of the new bone. Implanted cells found in the new bone stained immunohistochemically for osteocalcin, indicating that they had differentiated in vivo into osteogenic cells.

CONCLUSIONS

This study demonstrates that cells derived from muscle tissue that have been genetically engineered to express BMP-2 elicit the healing of critical-sized skull defects in mice. The cells derived from muscle tissue appear to enhance bone-healing by differentiating into osteoblasts in vivo.

CLINICAL RELEVANCE

Ex vivo gene therapy with muscle-derived cells that have been genetically engineered to express BMP-2 may be used to treat nonhealing bone defects. In addition, muscle-derived cells appear to include stem cells, which are easily obtained with muscle biopsy and could be used in gene therapy to deliver BMP-2.

摘要

背景

表达骨形态发生蛋白-2(BMP-2)的细胞现在可以通过用含有BMP-2 cDNA的腺病毒转导来制备。骨骼肌组织含有在BMP-2刺激下分化为成骨细胞的细胞。本研究的目的是通过用含有BMP-2 cDNA的腺病毒转导这些细胞来制备表达BMP-2的肌肉衍生细胞,并确定表达BMP-2的肌肉衍生细胞是否能促进小鼠临界尺寸骨缺损的愈合。

方法

用编码重组人BMP-2基因的腺病毒(adBMP-2)转导来自正常雄性小鼠的肌肉衍生细胞的原代培养物。将这些细胞(5×10⁵)植入雌性SCID(严重联合免疫缺陷品系)小鼠直径5毫米的临界尺寸颅骨缺损中,使用胶原海绵作为支架。在两周和四周时对治疗组和对照组的愈合情况进行大体和组织学检查。使用Y染色体特异性荧光原位杂交(FISH)技术在体内鉴定植入的细胞,并通过骨钙素免疫组织化学证明其向成骨细胞的分化。

结果

用经基因工程改造以表达BMP-2的肌肉细胞治疗的颅骨缺损在两周内闭合率>85%,在四周内闭合率为95%至100%。未治疗缺损的对照组(第1组)、仅用胶原治疗的对照组(第2组)或用胶原和不含adBMP-2的肌肉细胞治疗的对照组(第3组)在四周时缺损闭合率最高为30%至40%,且这些组中的大多数颅骨缺损未愈合。用Y染色体特异性FISH技术分析第4组中注射的细胞表明,大多数移植细胞位于新形成骨的表面,但一小部分(约5%)在新骨的骨细胞陷窝内被鉴定出来。在新骨中发现的植入细胞经骨钙素免疫组织化学染色,表明它们在体内已分化为成骨细胞。

结论

本研究表明,经基因工程改造以表达BMP-2的肌肉组织衍生细胞能促进小鼠临界尺寸颅骨缺损的愈合。肌肉组织衍生的细胞似乎通过在体内分化为成骨细胞来增强骨愈合。

临床意义

用经基因工程改造以表达BMP-2 的肌肉衍生细胞进行体外基因治疗可用于治疗不愈合的骨缺损。此外,肌肉衍生细胞似乎包括干细胞,通过肌肉活检很容易获得,可用于基因治疗以递送BMP-2。

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