Sherman L A, Lee J
Blood. 1982 Sep;60(3):558-63.
Plasma fibronectin (FN) binds fibrin in vitro by both noncovalent and covalent bonds and is decreased in DIC. In rabbits, conventionally purified 125I-FN had a complex blood clearance with a late t1/2 of 71 hr. A large portion was apparently altered, as evinced by rapid clearance and an intravascular/total body ratio (C1) of 0.28-0.51. 3H-labeled FN, made in vivo by injection of 3H amino acids, had a t1/2 of 73 hr. Crosstransfusion of 131I-FN and 3H-FN into a second set of animals gave similar t1/2s and C1s of 0.74-0.82, indicating the altered 125I-FN was biologically screened in the first animals. Other animals were given 125I-fibrinogen and "screened" 131I-FN. Intravenous thrombin (50-60 U/kg/1 hr) caused a 25%-50% decrease in both 125I-fibrinogen and 131I-FN. Ancrod injection reduced fibrinogen by greater than 90% but had no effect on 131I-FN. 131I-FN levels did not change when thrombin was given after ancrod. No cross-linked FN-fibrinogen alpha-chain was found in the plasma, nor was the thrombin-induced fall in FN affected by spermidine blockade. These experiments demonstrate that FN and fibrin bind in vivo during defibrination and are rapidly cleared from the blood. The abnormal fibrin resulting from ancrod either does not bind FN in vivo or does so reversibly.
血浆纤连蛋白(FN)在体外通过非共价键和共价键与纤维蛋白结合,在弥散性血管内凝血(DIC)时会减少。在兔子中,常规纯化的125I-FN具有复杂的血液清除率,其后期半衰期为71小时。很大一部分显然发生了改变,快速清除率和血管内/全身比率(C1)为0.28 - 0.51就证明了这一点。通过注射3H氨基酸在体内产生的3H标记的FN,半衰期为73小时。将131I-FN和3H-FN交叉输注到第二组动物中,得到了相似的半衰期和0.74 - 0.82的C1值,表明在第一组动物中改变的125I-FN经过了生物学筛选。给其他动物注射125I-纤维蛋白原和“筛选过的”131I-FN。静脉注射凝血酶(50 - 60 U/kg/1小时)导致125I-纤维蛋白原和131I-FN均降低25% - 50%。注射安克洛酶可使纤维蛋白原减少超过90%,但对131I-FN没有影响。在注射安克洛酶后再给予凝血酶时,131I-FN水平没有变化。血浆中未发现交联的FN-纤维蛋白原α链,精胺阻断也不影响凝血酶诱导的FN下降。这些实验表明,在去纤维蛋白过程中,FN和纤维蛋白在体内结合,并迅速从血液中清除。安克洛酶产生的异常纤维蛋白要么在体内不与FN结合,要么是可逆结合。
