Acquired coagulation dysfunction resulting from vitamin Kdependent coagulation factor deficiency associated with rheumatoid arthritis: A case report

BACKGROUND Rheumatoid arthritis(RA)is a common chronic inflammatory autoimmune disease with the main clinical feature of progressive joint synovial inflammation,which can lead to joint deformities as well as disability.RA often causes damage to multiple organs and systems within the body,including the blood hemostasis system.Few reports have focused on acquired coagulation dysfunction resulting from vitamin K-dependent coagulation factor deficiency associated with RA.CASE SUMMARY A 64-year-old woman with a history of RA presented to our hospital,complaining of painless gross hematuria for 2 wk.Blood coagulation function tests showed increased prothrombin time,international normalized ratio,and activated partial thromboplastin time.Abnormal blood coagulation factor(F)activity was detected(FII,7.0%;FV,122.0%;and FX,6.0%),indicating vitamin K-dependent coagulation factor deficiency.Thromboelastography and an activated partial thromboplastin time mixed correction experiment also suggested decreased coagulation factor activity.Clinically,the patient was initially diagnosed with hematuria,RA,and vitamin K-dependent coagulation factor deficiency.The patient received daily intravenous administration of vitamin K120 mg,etamsylate 3 g,and vitamin C 3000 mg for 10 d.Concurrently,oral leflunomide tablets and prednisone were administered for treatment of RA.After the treatment,the patient's symptoms improved markedly and she was discharged on day 12.There were no hemorrhagic events during 18 mo of follow-up.CONCLUSION RA can result in vitamin K-dependent coagulation factor deficiency,which leads to acquired coagulation dysfunction.Vitamin K1 supplementation has an obvious effect on coagulation dysfunction under these circumstances.

Treatment of vitamin K-dependent coagulation factor deficiency and subarachnoid hemorrhage

BACKGROUND： In adults, vitamin K-dependent coagulation factor deficiency （VKCFD） increases in the recent years. We treated a VKCFD patient with subarachnoid hemorrhage, with favorable outcomes.METHODS： A 19-year-old male student with VKCFD was treated at our hospital. The initial treatment was injection of a large dose of vitamin K and fresh plasma, and then with oral high dose of vitamin K4.RESULTS： At 4 weeks after admission, the focus of hemorrhage subsided, neurological examination was normal, and the patient was discharged.CONCLUSIONS： VKCFD is rare and its diagnosis should be based on the history of the patient and the results of laboratory examinations. A large dose of vitamin K is the fi rst choice of treatment.

Binding of EGF1 Domain Peptide in Coagulation Factor Ⅶ with Tissue Factor and Its Implications for the Triggering of Coagulation

The binding function of EGF1 domain peptide with tissue factor(TF)and its ability of triggering coagulation were explored.The TF expression model in vitro was established by lipopolysaccha-ride induction.The affinity of EGFP-EGF1 and TF expressing cells was analyzed by fluorescence microscopy and flow cytometry(FCM).The affinity of EGFP-EGF1 and rat soluble TF was quantitated by surface plasmon resonance(SPR).The ability of EGFP-EGF1 in triggering coagulation was tested by prothrombin time assay.The FCM res...

High-yield expression of recombinant mouse coagulation factor Ⅶ in methylotrophic yeast Pichia pastoris

Objective: To explore high-yield secretory expression of recombinant mouse coagulation factor Ⅶ (rmF Ⅶ ) protein in Pichia pastoris (P. pastoris). Methods: The fragment of mF Ⅶ cDNA was amplified by PCR from a pcDNA3-mFⅦ plasmid. Then the cDNA fragment was subcloned into α-factor secretion signal open reading frame of pPIC9K secretory expression vector. The mutagenesis of mF Ⅶ was performed by Site-Direct Mutation and then verified by DNA sequencing. The yeast expression vector of rmF Ⅶ, named as pPIC9K-rmFⅦ, was linearized with Sac I and transferred into GS115 strains(his-Mut+)by electroporation. The recombinants were identified by direct PCR and selection on MM and MD plates. rmF Ⅶ was expressed in recombinant strains (his+Mut+) for 4 d. The expression level and activation of rmF Ⅶ in the BMMY medium were detected by SDS-PAGE and Western blot respectively. Results:pPIC9K-rmFⅦ was constructed and transferred to GS115 strains successfully. 48-hour post induction by methanol rmFⅦ protein was secreted into the culture supernatant. The molecular weight of the expressed products was shown to be about 46 kD by SDS-PAGE analysis. Western blot showed that the expressed rmF Ⅶ exhibited specificity and antigenicity. Conclusion: Since mFⅦ is considered as a tumor-targeting molecule , this study may provide a basis for further anti-tumor strategy on rmFⅦ.

Relationship between Acquired Deficiency of Vitamin K-dependent Clotting Factors And Hemorrhage

This study examined the changes of activities of vitamin K-dependent clotting factors(VKDCF) under various pathological conditions and explored the relationship between acquired deficiency of VKDCFs and hemorrhage.Clinical data of 35 patients who were diagnosed as having acquired deficiency of VKDCF were retrospectively analyzed.Coagulation factors involved in the intrinsic and extrinsic pathways were detected in these patients and 41 control subjects.The results showed that the average activities of VKDCFs were decreased in the patients in comparison to the control subjects and significantly increased after treatment of these patients with vitamin K and blood products.Multivariate regression analysis indicated that decreased activity of VKDCF was not an independent risk factor for bleeding disorders owing to deficiency or metabolic disturbance of vitamin K.It was concluded that acquired deficiency of VKDCF occurs under a variety of pathologic conditions and is closely associated with hemorrhagic events.Administration of vitamin K and transfusion of blood products containing high concentrations of VKDCFs helps alleviate the hemorrhagic diseases.

冠心病血瘀证凝血因子Ⅶ基因多态性的检测分析

目的探讨凝血因子Ⅶ(FⅦ)基因多态性与冠心病(CHD)心血瘀阻证候及凝血因子Ⅶ活性(FⅦc)的相关性。方法对CHD心血瘀阻证组112例、非心血瘀阻证组108例、非CHD心血瘀阻证组110例和健康对照组100名检测分析FⅦ基因型(M1M1、M1M2、M2M2)和等位基因(M1、M2)及FⅦc。结果CHD心血瘀阻证组在基因型M1M1和等位基因M1频率分布均显著高于健康对照组(P<0.05);FⅦ-M1M1基因型的各组受检者FⅦc值的变化呈CHD心血瘀阻证组>非CHD血瘀证组>CHD非血瘀证组>健康对照组递减趋势;而FⅦ-M1M2基因型各组受检者FⅦc值的变化相反,呈现健康对照组<CHD非血瘀证组<非CHD心血瘀阻证组<CHD心血瘀证组的趋势;在三个病变组内,FⅦ基因M1M1型的FⅦc检测值均较M1M2型显著增高。结论FⅦ基因M1M1多态性和M1等位基因与CHD心血瘀阻证相关;FⅦ基因多态性与血浆Ⅶc密切相关。

尿毒症患者凝血因子Ⅶ水平及其影响因素

本研究检测慢性肾功能衰竭尿毒症期患者血浆凝血因子Ⅶ (FⅦ )水平并初步探讨其影响因素。选取 3 0例慢性肾功能衰竭尿毒症期患者 ,采用一期凝血法分别检测血液透析前及血液透析 1月后血浆凝血因子Ⅶ水平∶因子Ⅶ活性 (FⅦ∶C) ;采用重组可溶性组织因子一期凝血法检测活化因子Ⅶ (FⅦa) ;采用酶联免疫吸附法检测因子Ⅶ抗原 (FⅦAg)。结果显示 :①尿毒症患者血液透析前FⅦa、FⅦ∶C和FⅦAg水平分别为 4 .0 0± 0 .86μg/L、( 14 8.5± 4 0 .4 ) %和 ( 99.8± 2 1.1) % ,健康对照则分别为 2 .77± 1.0 2 μg/L、( 113 .1± 3 3 .0 ) %和 ( 73 .7± 18.3 ) % ,尿毒症患者的FⅦa ,FⅦ∶C ,FⅦAg水平与健康对照比较显著增高 (P 值均 <0 .0 5 ) ;②尿毒症患者血液透析后FⅦa,FⅦ∶C和FⅦAg水平分别为 5 .5 6± 1.4 5 μg/L、( 2 0 0 .8± 68.7) %和 ( 12 4 .1± 19.3 ) % ,与血液透析前相比较 ,FⅦa,FⅦ∶C和FⅦAg水平均显著增高 ( P值均 <0 .0 5 ) ;③尿毒症患者血液透析前FⅦAg ,FⅦ∶C及FⅦa水平与血尿素氮水平呈正相关 (相关系数分别为r =0 .3 7,P <0 .0 5 ;r =0 .4 0 ,P <0 .0 5 ;r =0 .2 8,P <0 .0 5 ) ;与血肌酐水平亦呈正相关 (相关系数分别为r =0 .14 ,P <0 .0 5 ;r =0 .2 3 ,P <0 .0 5 ;r =0 .18。

10例遗传性凝血因子Ⅶ缺陷症分子发病机制与临床特性分析

目的 探讨 10例遗传性凝血因子Ⅶ (coagulationfactorⅦ ,FⅦ )缺陷症基因突变类型与临床特性。方法 检测凝血指标以明确诊断 ;用DNA直接测序法对先证者及其家庭成员FⅦ基因的全部外显子及其侧翼、5’和 3’非翻译区进行分析 ,寻找基因突变 ;将含插入或缺失突变序列克隆入pMD18 TTA克隆载体中 ,对所得两条染色体相应序列分别测序 ,以确定突变在染色体上的分布。应用限制性内切酶对先证者及家系成员相应基因片段进行酶切分析 ,无酶切位点改变的基因片段用等位基因特异的PCR(ASPCR)方法 ,证实测序所发现的突变。结果 在 10例遗传性凝血因子Ⅶ缺陷症患者中发现 8种类型的基因突变 ,其中 6 390T→C(Phe4 0Cys) ,94 82G→T(Arg15 2Leu) ,和 114 87 9delC 3种突变为国际首次报道 ;6种突变发生在催化区 ;除一种缺失突变外 ,其余均为点突变 ;所有的基因突变都来自先证者的父亲和 (或 )母亲。Thr35 9Met和Arg30 4Trp突变分别在 4个及 2个无亲缘关系的家系中重复出现。 2例Thr35 9Met纯合突变 (FⅦ :C分别为 2 %和 3% )及 1例Arg15 2Leu、114 87 9delC及Arg30 4Trp复合杂合突变 (FⅦ :C为 1% )临床表型为重型 ;2例双重杂合突变 (His348Gln和Thr35 9Met,Agr30 4Trp和Arg30 4Gln)临床表型分别为中型和无症状

不同温度和时间对凝血因子Ⅶ的影响

目的 探讨不同温度、时间条件下血浆凝血因子Ⅶ (FⅦ )活性的变化 ,以探寻检测FⅦ活性的最适条件。方法 凝血因子活性测定采用一步法检测血浆FⅦ :C活性水平及相应的凝血酶元时间 (PT)。将标本分别置于 0℃、2 2℃环境中 ,1、2、4小时上机检测。结果 0℃ 4小时与 0℃ 1小时、2小时 ,检测FⅦ :C活性水平差异有显著性意义 (P <0 .0 5 ) ;2 2℃ 1、2、4小时检测FⅦ :C活性水平差异有显著性意义 (P <0 .0 5 ) ;2 2℃ 1小时与 0℃ 2小时检测FⅦ :C活性水平差异无显著性意义 (P >0 .0 5 )。结论 0℃条件下血浆FⅦ可被激活 ,但在 2小时内对凝血时间测定影响不大 ,故不能及时检测的患者血样应在 2小时内用冰水保存。

凝血因子Ⅶ基因突变的检测

目的 为检测福建省福州市一个遗传性凝血因子缺乏症先证者的因子Ⅶ基因突变类型。方法 采有ＰＣＲ结合限制性内切酶ＨｇｉＣＩ，以先证者及其母亲的 ＦⅦ基因片进行分析。结果表明先证者的 ＦⅦ基因为 Ｃ３２９Ｇ纯合子，其母亲为杂合子。结论 该家系为ＦⅦ基因存在Ｃ３２９Ｇ突变的第２个遗传性因子Ⅶ缺乏症家系。

河南汉族深静脉血栓形成患者凝血因子Ⅶ基因多态性检测

目的:检测河南汉族深静脉血栓形成(DVT)患者凝血因子Ⅶ(FⅦ)基因的多态性。方法:采用聚合酶链反应-限制性片段长度多态性方法检测103例河南汉族DVT患者和250名正常对照者FⅦ基因R353Q、5’F7和IVS7位点的多态性,并进行基因型频率、等位基因频率的比较及单倍型分析。结果:DVT组和对照组R353Q、5’F7基因型频率及等位基因频率差异无统计学意义(P均>0.05);2组IVS7基因型频率差异亦无统计学意义(χ2=0.327,P=0.569),DVT组H7等位基因频率(44.7%)低于对照组(51.8%)(χ2=4.112,P=0.043)。结论:FⅦ基因R353Q、5’F7多态性可能不是河南汉族人群DVT发病的遗传学风险因子;IVS7多态的H7等位基因可能是河南汉族人群DVT发病的遗传保护因子。

凝血因子Ⅶ及其基因MspI多态性与心肌梗塞危险性的研究

目的；探讨凝血因子Ⅶ活性及其基因ＭｓｐＩ多态性与中国汉族人心肌梗塞的关系。 方法：测定１２５例健康人（正常对照组）和１３７例心肌梗塞患者（心肌梗塞组）血浆凝血因子Ⅶ活性；采用聚合酶链反应（ＰＣＲ）和ＭｓｐＩ酶切法确定其基因型。 结果：①心肌梗塞组血浆凝血因子Ⅶ活性（Ｐ＜０．０１）和血清总胆固醇（Ｐ＜０．０５）均显著高于正常对照组；仅前者与心肌梗塞的危险性独立相关（ＯＲ＝１．０４，Ｐ＜０．０１）。②凝血因子Ⅶ基因型和等位基因的频率分布在两组间无显著差异。③Ｍ_１Ｍ_１纯合子血浆凝血因子Ｗ活性显著高于Ｍ_１Ｍ_２杂合子（Ｐ＜０．０５）。 结论：支持血浆凝血因子Ⅶ活性升高是中国汉族人心肌梗塞的危险因素；凝血因子Ⅶ活性受其基因ＭｓｐＩ多态性的影响，但该多态性并不是中国汉族人心肌梗塞的独立危险因子。

河南汉族缺血性脑卒中患者凝血因子Ⅶ基因R353Q多态性检测

目的探讨河南汉族人群缺血性脑卒中患者凝血因子Ⅶ(FⅦ)基因R353Q的多态性。方法应用PCR-限制性片段长度多态性(PCR-RFLP)分析技术,检测560例健康对照组和512例缺血性脑卒中患者FⅦ基因R353Q多态性。结果FⅦ基因第353位存在R、Q2种等位基因,以及R/R、R/Q和Q/Q3种基因型。患者组Q等位基因频率和R/Q+Q/Q型频率低于正常对照组(P<0.05)。结论河南汉族人群中存在凝血因子Ⅶ基因R353Q多态性,其中Q等位基因可能是缺血性脑卒中的遗传保护因子。

凝血因子Ⅶ及其基因MspI多态性与高血压合并脑梗死的相关性

探讨血浆活化凝血因子Ⅶ及其基因MspI多态性与中国汉族人高血压合并脑梗死的关系。采用侯选基因及病例—对照的方法 ,以聚合酶链反应及限制性内切酶片段长度多态性分析技术 ,对高血压组、高血压合并脑梗死组及正常对照组进行凝血因子Ⅶ基因MspI多态性分析并确定基因型 ,同时采用重组可溶性组织因子法测定血浆活化凝血因子Ⅶ水平。结果发现 ,与高血压组比较 ,脑梗死组血浆活化凝血因子Ⅶ水平显著增高 (2 .78± 0 .5 9比2 .5 3± 0 .6 2 μg L ,P <0 .0 5 ) ;高血压组与正常对照组比较差异无显著性 (2 .5 3± 0 .6 2比 2 .4 1± 0 .6 1μg L ,P >0 .0 5 ) ;Logistic回归分析显示 ,血浆活化凝血因子Ⅶ水平增高是高血压合并脑梗死的重要危险因素 (OR =1.134,P <0 .0 5 ) ;凝血因子Ⅶ基因型频率分布符合Hardy Weinberg平衡定律 ,基因型及等位基因频率分布在各组间差异均无显著性 (P >0 .0 5 ) ;各组血浆活化凝血因子Ⅶ水平均与凝血因子Ⅶ基因多态性显著相关 ,M1 M1 纯合子血浆活化凝血因子Ⅶ水平显著高于M2 等位基因携带者 (P <0 .0 5 )。以上提示 ,血浆活化凝血因子Ⅶ水平增高是高血压合并脑梗死的重要危险因素 ,并受其基因MspI多态性的影响。

慢性乙型肝炎伴凝血因子Ⅶ缺乏1例并文献复习

目的复习慢性乙型肝炎合并遗传性凝血因子Ⅶ缺乏的特点。方法分析1例慢性乙型肝炎伴遗传性凝血因子Ⅶ缺乏症患者的临床资料,并复习相关文献。结果该患者PT明显延长,FⅦ活性降低,而APTT及其他凝血因子活性均正常,HBV标记物阳性,而肝功能指标正常。结论遗传性凝血因子Ⅶ缺乏症是临床上一种非常少见的出血性疾病,多伴有基因缺陷,目前尚无根治的方法。对于慢性乙型肝炎患者PT明显延长而肝功能正常时,应积极查找肝病以外的原因。

遗传性凝血因子Ⅶ缺乏症研究进展

遗传性凝血因子Ⅶ(FⅦ)缺乏症是一种在临床上非常少见的出血性疾病,常与FⅦ基因缺陷有关,其临床表型往往与FⅦ基因的突变类型及突变区域密切相关。近年来国际上相继进行了几个较大的遗传性FⅦ缺乏症相关研究的合作项目,发现了新的基因突变,丰富了疾病相关基因突变数据库,而且在疾病基因治疗方面也取得了可喜的进展。

重组小鼠凝血因子Ⅶ毕赤酵母表达载体的构建及整合体的筛选

目的构建无凝血活性的重组小鼠凝血因子Ⅶ(rmFⅦ)毕赤酵母分泌型表达载体,获得高拷贝稳定整合菌株,为大量获得rmFⅦ蛋白,进行功能研究及其临床应用奠定基础。方法PCR扩增得到mFⅦ基因片段,插入酵母表达载体pPIC9K的α分泌信号开放阅读框的下游,再经定点突变(K341A)得到pPIC9KrmFⅦ,测序正确的质粒用SacⅠ线性化后电穿孔转化毕赤酵母GS115,G418梯度筛选转化菌,PCR鉴定目的基因的整合。结果获得了rmFⅦ毕赤酵母表达载体pPIC9KrmFⅦ,G418抗性筛选得到高拷贝菌株,PCR证实目的基因已整合到毕赤酵母染色体中。结论成功构建了rmFⅦ毕赤酵母表达载体,获得了高拷贝稳定整合菌株,为大规模表达纯化rmFⅦ蛋白及后续研究奠定了基础。

凝血因子Ⅶ C329G突变导致遗传性凝血因子Ⅶ缺乏症

目的探讨遗传性凝血因子Ⅶ缺乏症发病的分子机制。方法将野生型和C329G突变型的FⅦ真核表达载体转染BHK-21细胞进行体外表达,并对表达产物进行免疫学和凝血活性检测。结果FⅦC329G突变后,其蛋白的合成和分泌不受影响,突变型与野生型FⅦ的表达量相近,但突变型FⅦ无凝血活性。结论FⅦ第329位的半胱氨酸对其凝血活性功能起关键作用。当它被甘氨酸替换后,即丧失其凝血活性,此为FⅦC329G突变导致遗传性凝血因子Ⅶ缺乏症发病的分子机制。

慢性重型肝炎凝血因子Ⅴ、Ⅶ、Ⅹ的动态变化及临床意义

探讨慢性重型肝炎患者血清中凝血因子Ⅴ、Ⅶ、Ⅹ水平的动态变化及临床意义。方法:78例慢性重型肝炎患者分为死亡组和存活组,前者分为早期、中期、晚期,后者分为早期、恢复期,采用血凝法动态检测两组各期及对照组中患者凝血因子Ⅴ、Ⅵ、Ⅹ的水平,并比较它们之间的差异。结果:慢性重型肝炎患者死亡组早期凝血因子Ⅴ、Ⅶ、Ⅹ水平分别为34.64±2.89、20.96±2.23、42.62±3.28,中期分别为22.81±2.28、14.40±1.63、32.67±2.70,晚期分别为14.25±1.76、9.90±1.48、25.76±2.44,均显著低于正常对照组,且随肝功能受损程度加剧而呈进行性降低,其中19因子下降最明显。存活组早期3种因子水平分别为45.58±8.69、21.96±6.61、42.27±12.25,均显著低地正常对照组。恢复期中Ⅶ因子为68.85±31.74,Ⅹ因子为64.12±11.65,仍低于正常对照组(P<0.05),但Ⅴ因子与对照组相比差异无显著性(P>0.05)。在存活组与死亡组的早期Ⅴ因子的活性有显著性差异(t=2.44,P<0.05),而Ⅶ因子、Ⅹ因子差异无显著性(t值分别为0.38、0.09,P>0.05)。结论:动态观察凝血因子Ⅴ、Ⅶ、Ⅹ水平的变化,对慢性重型肝炎的早期诊断和判断预后有一定价值。Ⅶ因子是较灵敏的指标,Ⅴ因子是判断预后的最好指标,由于凝血酶原时间(PT)和凝血酶原活动度(PTA)

可溶性血管细胞黏附分子-1及凝血因子Ⅶ与脑梗死的相关性研究

目的分析可溶性血管细胞黏附分子-1（soluble vascular cell adhesion molecule-1，sVCAM-1）与凝血因子Ⅶ（coagulation factor Ⅶ，FⅦ）与脑梗死发生、发展的相关性。方法分别采用双抗体夹心ABC—ELISA法和全自动血凝仪CASOO的一阶段凝固法动态检测30例急性脑梗死患者血清sVCAM-1及血浆FⅦ：C水平，以26例脑动脉供血不足患者和30例健康老年人为对照组。结果血清sVCAM-1水平在脑梗死发生第1d显著高于脑供血不足对照组和正常人对照组（P〈0．01），1-7d呈增高趋势，7～14d呈下降趋势。脑梗死体积越大，sVCAM-1水平越高（P〈0．01）。脑梗死患者血浆FⅦ：C水平两对照组无统计学差异（P〉0．05）。结论sVCAM-1与急性脑梗死密切相关，与脑梗死的发生、发展有一定的联系，可用作脑梗死病程进展的监测指标。FⅦ与急性脑梗死的发生及进程均无显著相关性。