Value of circulating cell-free DNA in diagnosis of hepatocelluar carcinoma

AIM:To investigate the value of combined detection of circulating cell-free DNA(cfDNA),a-fetal protein(AFP) and a L-fucosidase(AFU) for diagnosis of hepatocellular carcinoma(HCC).METHODS:Serum samples from 39 HCC patients and 45 normal controls were collected.Branched DNA(bDNA) was used to detect the level of cfDNA,and a receiver operating characteristic curve was employed to evaluate the diagnostic sensitivity,specificity,accuracy,positive predictive value,negative predictive value,positive likelihood ratio,negative likelihood ratio and Youden index,and to assess the diagnostic efficiency and their correlations with the clinicopathological features.AFP and AFU were detected by chemiluminescence and colorimetry,respectively.The significance of combined detection of the three biomarkers was discussed.RESULTS:cfDNA level was increased in 22 of the 39 HCC samples and in 2 of the 45 normal controls.cfDNA level in HCC samples was significantly higher than that in normal controls(P < 0.05).There were significant differences in sex and extra-and intrahepatic metastasis(P < 0.05).There was no significant correlation between cfDNA,AFP and AFU in the detection of HCC.The sensitivity of combined detection of cfDNA with one marker(AFP or AFU) and cfDNA with two markers(AFP and AFU) was 71.8%,87.2% and 89.7% vs 56.4%,53.8% and 66.7% for cfDNA,AFP and AFU used alone,respectively,the difference being statistically significant(P < 0.05).CONCLUSION:Quantitative analysis of cfDNA is sensitive and feasible,and the combined detection of cfDNA with AFP or AFU or both could improve the diagnostic sensitivity for HCC.

Prognostic and predictive blood biomarkers in gastric cancer and the potential application of circulating tumor cells

Gastric cancer(GC), with its high incidence and mortality rates, is a highly fatal cancer that is common in East Asia particularly in China. Its recurrence and metastasis are the main causes of its poor prognosis. Circulating tumor cells(CTCs) or other blood biomarkers that are released into the circulating blood stream by tumors are thought to play a crucial role in the recurrence and metastasis of gastric cancer. Therefore, the detection of CTCs and other blood biomarkers has an important clinical significance; in fact, they can help predict the prognosis, assess the staging, monitor the therapeutic effects and determine the drug susceptibility. Recent research has identified many blood biomarkers in GC, such as various serum proteins, autoantibodies against tumor associated antigens, and cell-free DNAs. The analysis of CTCs and circulating cell-free tumor DNA(ctDNA) in the peripheral blood of patients with gastric cancer is called as liquid biopsy. These blood biomarkers provide the disease status for individuals and have clinical meaning. In this review, we focus on the recent scientific advances regarding CTCs and other blood biomarkers, and discuss their origins and clinical meaning.

磁共振动态增强结合血循环肿瘤细胞、循环游离DNA对乳腺癌的临床诊断研究

目的探讨磁共振动态增强(DCE-MRI)结合血循环肿瘤细胞(CTCs)、循环游离DNA(cfDNA)对乳腺癌的诊断价值。方法选取沧州市人民医院2020年6月至2021年11月符合纳入标准的乳腺癌病人82例(乳腺癌组)。另选同期65例乳腺良性病变且未合并其他疾病者作为良性组。比较两组DCE-MRI定量参数、CTCs、cfDNA水平,对比MRI特征,分析DCE-MRI结合CTCs、cfDNA诊断乳腺癌的价值。结果乳腺癌组DCE-MRI定量参数速度常数(K^(trans))值、速率常数(K_(ep))值、Alu247/115水平及CTCs计数分别为(0.18±0.04)min、(1.32±0.27)min、(12.97±2.14)个/毫升、0.97±0.32,比良性组高(0.05±0.01)min、(0.51±0.11)min、(10.15±1.45)个/毫升、0.55±0.12(P<0.05)。良性组边缘多光滑,形状规则,内部强化以均匀为主,时间-信号强度曲线(TIC)以Ⅰ型多见,早期增强率<60%;乳腺癌组边缘毛刺征、形状不规则,内部不均匀强化为主,以TIC分型Ⅲ型多见,早期增强率<60%占比高。两组MRI形态表现比较差异有统计学意义(P<0.05)。淋巴结转移、Ⅲ~Ⅳ期者CTCs数量、Alu247/115水平明显高于无淋巴结转移、Ⅰ~Ⅱ期者(P<0.05)。受试者操作特征(ROC)曲线分析结果显示,三者联合(DCE-MRI+CTCs+cfDNA)诊断乳腺癌的曲线下面积(AUC)、灵敏度、特异度分别为0.86、0.93、0.84,诊断效果优于单一检测CTCs、cfDNA检测(P<0.05)。结论乳腺癌病人CTCs、cfDNA存在异常表达,可能与病人临床分期、淋巴结转移有关,相对单一实验室检测,DCE-MRI结合CTCs、cfDNA检测能获取更多可靠信息。

The Prognostic Value of Cell-Free DNA in Advanced Non-Small-Cell Lung Cancer

Background: Cell-free DNA (cfDNA) holds promise as a tumor marker of clinical importance. We aimed to investigate the prognostic value of baseline cfDNA in non small-cell lung cancer (NSCLC). Material and Methods: During a three-year period, patients with newly diagnosed, previously untreated advanced NSCLC were included in a consecutive, prospective marker-trial. Plasma was isolated from a pre-treatment peripheral blood sample and the level of total cfDNA was measured by an in-house assay qPCR-method. The treatment comprised carboplatin (AUC 5) intravenously day 1), and vinorelbine (30 mg/m2 intravenously day 1 and 60 mg/m2 perorally day 8) q3w for a maximum of six cycles. The primary end-point was overall survival (OS). Secondary end-points were progression free survival (PFS) and overall response rate (ORR). Results: 245 patients were included and received a minimum of 1 cycle of chemotherapy (median 4). The median OS was 8.9 months, the median PFS by intention to treat 5.4 months and the ORR was 25%. The patients were divided into four groups based on quartiles of cfDNA and subsequently dichotomized by the 75th percentile revealing a significantly worse prognosis for patients in the upper 75th percentile (median OS 4.9 months) compared to patients with lower levels (10.0 months) (HR 2.1, 95%CI 1.4 - 3.1, p 0.0001). A multivariate analysis confirmed the independent prognostic value of cfDNA. A subgroup analysis of patients with high cfDNA and poor performance status (PS = 2) identified a group of patients with even worse prognosis (median OS 2.0 versus 9.1 months, HR 3.6, 95%CI 1.4 - 9.2, p 0.0001). Similar and significant results were found when comparing level of cfDNA and PFS. Conclusions: High pre-treatment level of cfDNA seems to have a strong prognostic impact in patients with newly diagnosed advanced NSCLC. Combined with PS it identifies a patient group with minimal or no benefit of chemotherapy.

DNA甲基化谱:流淌的生命脉律——纪念DNA双螺旋结构发现70周年

70年前,随着DNA双螺旋结构的发现,人类进入基因组时代;21世纪初,人类基因组测序完成及对转录组、蛋白质组和表观遗传的研究,人类继而进入后基因组时代;近年对DNA甲基化的深入研究,预示更为神秘宽广的表观遗传组学时代已经到来。人体血液中大量存在的甲基化DNA构成甲基化谱,作为一个整合性指标,有如一曲流淌的生命脉律,反映不同细胞的生理或病理状态。精准分析甲基化谱,具有诊断疾病特别是肿瘤早筛早诊的价值;同时可作为人类健康、乃至天赋的量化评估指标;也可用于中医体质辨识与证型分类及中药材溯源、真伪识别和品种改良。本文介绍表观遗传组学时代甲基化谱的重要意义,以纪念DNA双螺旋结构发现70周年。

转移性结直肠癌cfDNA的早期动态变化与一线化疗疗效的相关性分析

目的探讨转移性结直肠癌患者一线化疗期间循环游离DNA(cfDNA)的早期动态变化与一线化疗疗效及预后的相关性。方法纳入南京医科大学附属肿瘤医院2018年7月至2020年4月接受一线化疗的118例转移性结直肠癌患者,对其血浆中的cfDNA进行定量检测。分析患者的cfDNA基线水平与临床特征、cfDNA动态变化与无进展生存期(PFS)及治疗反应之间的相关性。结果患者的病理类型、有无肝转移、原发灶位置的不同分组间cfDNA水平差异有统计学意义(P<0.05)。而4周期化疗后cfDNA比值(化疗后cfDNA水平/cfDNA基线水平)≤1.215的患者PFS更长,客观缓解率(ORR)更高。通过多变量Cox回归分析,我们还发现一线化疗4周期后cfDNA比值是晚期结直肠癌患者一线化疗的独立预后因素。结论转移性结直肠癌cfDNA的基线水平与肿瘤侵袭性、肿瘤负荷相关,一线化疗期间cfDNA的早期动态变化可有效预测一线化疗疗效及预后。

ccfDNA中RERG甲基化状态检测在诊断鼻咽癌中的临床意义

目的研究循环细胞游离DNA(ccfDNA)中RAS样雌激素调节生长抑制因子(RERG)基因甲基化状态检测在诊断鼻咽癌中的临床意义。方法选取2020年1月至2021年6月在该院就诊的100例(病理学诊断)原发性鼻咽癌患者作为鼻咽癌组,同时选取97例非癌志愿者作为对照组。提取活检组织DNA和ccfDNA,通过实时荧光定量PCR法DNA甲基化分析(qAMP)检测组织DNA和ccfDNA中RERG mRNA甲基化率。绘制受试者工作特征(ROC)曲线评价ccfDNA中RERG mRNA甲基化率对鼻咽癌的诊断价值。结果基于TCGA数据库中来自于头颈部鳞状细胞癌(HNSC)组织标本的RNA-Seq转录本数据相应患者临床资料,HNSC组织标本中RERG mRNA表达明显低于正常组织,RERG mRNA甲基化β值高于正常组织(P<0.001)。在临床试验中,鼻咽癌组ccfDNA中RERG mRNA甲基化率高于对照组[0.127(0.095,0.175)vs.0.023(0.014,0.036),P<0.001]。经ROC曲线分析,检测ccfDNA中RERG mRNA甲基化率诊断鼻咽癌的曲线下面积(AUC)为0.990(95%CI:0.980~0.999)。ccfDNA和肿瘤组织中RERG mRNA甲基化率呈正相关(r=0.407,P<0.001)。鼻咽癌患者ccfDNA中RERG mRNA甲基化率在不同肿瘤T分期、N分期、TNM分期及EB病毒(EBV)DNA状态人群之间差异有统计学意义(P<0.05)。结论ccfDNA中RERG mRNA甲基化状态可能为鼻咽癌筛查中潜在的血液学生物标志物。

血清循环游离DNA与类风湿关节炎患者临床指标的关系

目的:研究循环游离DNA(cell-free DNA,cfDNA)在类风湿关节炎(rheumatoid arthritis,RA)患者外周血中含量对RA早期诊断和疾病活动度的评估价值,探讨cfDNA含量与RA的免疫学诊断指标及疾病活动度评估的相关指标类风湿因子(rheumatoid factor,RF)、抗环瓜氨酸抗体(anti-cyclic citrullinated peptide antibodies,抗CCP抗体)、C反应蛋白(C-reactive protein,CRP)、红细胞沉降率(erythrocyte sedimentation rate,ESR)和28个关节疾病活动指数评分(disease activity score of 28 joints,DAS28-ESR)间的关系。方法:收集80例初诊且未接受抗风湿类药物治疗的RA患者为观察组(RA组),40例健康人为对照组(HC组),收集两组血清,测定cfDNA含量并计算完整度,与收集的RA患者临床指标进行相关性分析。结果:RA组的cfDNA高于HC组(P<0.05),但与诊断性血清学指标不相关(P>0.05)。根据28个关节疾病活动指数评分(DAS28-ESR评分)对RA患者进行疾病活动度分层,发现cfDNA含量在DAS28-ESR评分高组高于评分低组(P<0.05),cfDNA与DAS28-ESR、CRP和ESR具有相关性(P<0.05)。结论:血清cfDNA在RA患者体内含量增加,与炎症反应有相关性,对RA有诊断价值,可能是RA致病的独立危险因素。

DNA methylation signatures in circulating cell-free DNA as biomarkers for the early detection of cancer

Detecting cell-free DNA(cfDNA) or circulating tumor DNA(ctDNA) in plasma or serum could serve as a "liquid biopsy", which would be useful for numerous diagnostic applications. cfDNA methylation detection is one of the most promising approaches for cancer risk assessment. Here, we reviewed the literature related to the use of serum or plasma circulating cell-free DNA for cancer diagnosis in the early stage and their power as future biomarkers.

Liquid biopsies:DNA methylation analyses in circulating cell-free DNA

Analysis of patient＇s materials like cells or nucleic acids obtained in a minimally invasive or noninvasive manner through the sampling of blood or other body fluids serves as liquid biopsies, which has huge potential for numerous diagnostic applications. Circulating cell-free DNA（cfDNA） is explored as a prognostic or predictive marker of liquid biopsies with the improvements in genomic and molecular methods. DNA methylation is an important epigenetic marker known to affect gene expression. cfDNA methylation detection is a very promising approach as abnormal distribution of DNA methylation is one of the hallmarks of many cancers and methylation changes occur early during carcinogenesis. This re？view summarizes the various investigational applications of cfDNA methylation and its oxidized de？rivatives as biomarkers for cancer diagnosis, prenatal diagnosis and organ transplantation monitoring.The review also provides a brief overview of the technologies for cfDNA methylation analysis based on next generation sequencing.

血浆游离DNA含量及其完整性检测对肝癌的诊断价值

目的比较实时荧光定量PCR(RT-PCR)对肝细胞癌(HCC)、乙型病毒性肝炎(简称乙肝)患者及健康体检者血浆游离DNA含量及完整性的检测结果,探讨实时荧光定量PCR(RT-PCR)对HCC的诊断价值。方法收集52例HCC患者、58例乙肝患者和60例健康体检者的静脉血标本,采用RT-PCR技术对各组血浆游离DNA中GAPDH、β-actin400、β-actin167含量及其完整性(β-actin400/β-actin167)进行定量检测,结果采用SPSS软件进行统计学分析。结果健康对照组的血浆游离DNAβ-actin167含量和完整性相比明显低于HCC组(Z=–4.328,P=0.000;Z=–3.885,P=0.001)和乙型肝炎病毒(HBV)组(Z=–2.473,P=0.005;Z=–3.295,P=0.013),且HBV组血浆游离DNA完整性明显低于HCC组(Z=–4.836,P=0.002)。结论 RT-PCR检测血浆游离DNA完整性(β-actin400/β-actin167)可作为HCC辅助诊断的分子生物学指标。

中性粒细胞胞外诱捕网与口腔鳞状细胞癌关系的 研究进展

中性粒细胞胞外诱捕网(neutrophil extracellular traps,NETs)是中性粒细胞释放的一种由解聚的染色质和颗粒蛋白组成的纤维网状结构,可以捕获和杀死细菌。NETs的形成由各种细菌、病毒等病原体激活,其过程被称为网捕死亡(NETosis)。NETosis是一种不同于细胞凋亡和细胞坏死的细胞程序性死亡过程,目前已经报道了两种NETosis形式:裂解性NETosis和非裂解性NETosis。研究发现NETs能够在肿瘤微环境(tumor microenvironment,TME)中与免疫细胞相互作用,激活巨噬细胞;促进髓系抑制细胞的免疫抑制作用;并能包裹在肿瘤表面,防止CD8+T细胞和自然杀伤细胞发挥细胞毒性作用。近年研究发现,NETs在口腔鳞状细胞癌(oral squamous cell carcinoma,OSCC)组织中大量存在,与OSCC发生发展关系复杂,根据不同的中性粒细胞表型,NETs可发挥促肿瘤或抗肿瘤作用,对N1型中性粒细胞,NETs可能是其发挥抗肿瘤作用的手段,而转换生长因子⁃β(transforming growth factor⁃β,TGF⁃β)诱导的NETs的形成可能与N2型中性粒细胞呈现促癌活性从而诱导口腔扁平苔藓恶变的机制有关。NETs还可能参与OSCC的转移过程,其通过捕获循环肿瘤细胞(circu⁃lating tumor cells,CTC)并诱导高凝状态促进肿瘤相关血栓的形成和血源性转移。NETs参与了OSCC发生和转移的过程,为抗肿瘤治疗和预测OSCC的预后提供了新的研究方向。抑制NETs的形成可以显著抑制化疗后产生的耐药性,并有利于降低OSCC患者的血栓形成风险从而抑制肿瘤转移。目前基于NETs相关基因已构建了多个关于头颈部鳞状细胞癌的预后模型。但目前NETs与OSCC的治疗尚处于讨论阶段,其作用机制与实行的可能性尚需大规模的基础与临床试验验证。本文通过综述NETs与OSCC之间的关系,为治疗OSCC提供新思路。

孕妇外周血中胎儿游离DNA在产前诊断中的应用

孕妇外周血中胎儿游离DNA的发现,为无创性产前诊断开辟了一条新途径。检测孕妇血浆中特异的胎儿DNA序列已被用于胎儿性连锁疾病鉴定、RhD血型检查和多种单基因遗传病的产前诊断;游离DNA水平的变化还可被用作某些妊娠相关疾病如先兆子、早产和胎儿染色体疾病的临床诊断新指标。本文对母体外周血中胎儿游离DNA的生化特征及其临床应用研究,进行了总结和分析。

循环游离DNA在乳腺癌中的临床应用

循环游离DNA以细胞外游离形式存在于血液中,可由正常细胞和癌细胞释放。乳腺癌患者血液中循环游离DNA水平高于正常人,且循环游离DNA可以反映癌组织的基因突变、甲基化状态、拷贝数改变、杂合子丢失等特征,是乳腺癌诊断、治疗、预后检测中具有巨大潜力的生物学指标。本综述简要介绍了循环游离DNA的生物学特性,并从定量及定性检测两方面对循环游离DNA近年来在乳腺癌中的临床应用进行较全面的阐述。

血循环DNA在淋巴瘤中的定量检测及其临床意义

目的:了解血循环DNA含量在淋巴瘤筛查中的应用价值,分析其与标准化疗方案治疗后治疗效果及预后的关系,探讨血循环DNA定量在淋巴瘤评估疗效及指导预后中的重要作用。方法:收集32例浅表淋巴结肿大的淋巴瘤者21例(标准化疗方案前后分别采集外周血标本)和淋巴结炎者11例的外周血标本。另选取9名健康志愿者的外周血标本作为健康对照组。使用荧光定量PCR方法检测各组标本的血循环DNA水平,分析血循环DNA在不同组别中的表达水平,了解其与淋巴瘤临床特征间的联系,评估血循环DNA清除率在治疗效果及预后判断中的重要作用。结果:淋巴瘤患者的血循环DNA水平均明显高于淋巴结炎者和健康志愿者(56.71±50.61)ng/ml vs(19.21±15.52)ng/ml和(8.26±7.06)ng/ml,(P=0.033和P=0.010),后两者间无统计学意义(P=0.118)。淋巴瘤患者血循环DNA与乳酸脱氢酶水平明显相关(P=0.032)。当血循环DNA水平24.67 ng/ml作为诊断淋巴瘤的临界值时,其敏感度为75%,特异度为85%。标准方案化疗结束后血循环DNA清除率高的患者,完全缓解率高(P=0.032),总生存期长(P<0.001)。结论:血循环DNA在淋巴瘤中明显增高,可能有助于淋巴瘤筛查。血循环DNA水平有可能作为淋巴瘤疗效判断及预后评估的一个潜在指标。

外周血液中循环肿瘤细胞和循环游离DNA检测在乳腺癌患者中的应用

目的探究外周血液中循环肿瘤细胞(CTCs)和循环游离DNA(cfDNA)检测在乳腺癌患者中的应用效果。方法收集本院2018-02—2019-02收治的94例乳腺癌患者、48例乳腺良性疾病患者及56例健康体检者外周血液标本,采用基于尺寸的高通量微流控芯片捕获CTCs、基于Alu序列的实时荧光定量PCR检测游离DNA长、短片段(247 bp、115 bp),并以长、短片段扩增产物比值作为DNA完整性指标。分析CTCs和cfDNA与乳腺癌临床参数的关系,并评估其在乳腺癌诊断中的作用。结果乳腺癌患者在CTCs、血浆cfDNA的基于Alu序列的Alu 247/115的比值上显著比健康体检者、乳腺良性疾病者高(P<0.05),乳腺癌患者外周血中CTCs的数量与血浆cfDNA的基于Alu序列的Alu 247/115的比值在年龄、病理分期、淋巴结转移、分子分型、远处转移、PR有一定的相关性(P<0.05),以病理学结果作为金标准,以约登指数最大点对应的临界值,以乳腺良性疾病患者和健康体检者作对照,当CTCs cut-off值为7.68个/ml,灵敏度为80.4%,特异度为96.4%,ROC曲线下面积为0.885(95%CI 0.805~0.965);Alu 247/115的cut-off值为0.431时,特异度为71.4%,ROC曲线下面积为0.727(95%CI 0.608~0.847),灵敏度为71.7%。结论 CTCs与cfDNA可能是乳腺癌辅助诊断的潜在生物学指标,CTCs检测的是肿瘤细胞,cfDNA检测的是肿瘤的DNA片段,可作为判断乳腺癌患者的病情变化和诊断的良好辅助指标,此方法值得应用与推广。

基于RASSF1A为标志的无损性孕妇血浆中胎儿RHD-DNA检测方法的建立

目的建立基于表观遗传标志RASSF1A为标志的孕妇外周血浆中胎儿RHD-DNA检测路径,用于无损性产前胎儿RhD血型预测。方法首先采用PCR-SSP对孕妇外周血细胞基因组DNA做RHD基因多个外显子检测,以确定其RHD基因型;其次对无外显子表达或部分外显子表达的孕妇,对其外周血浆中胎儿游离的DNA采用RTPCR扩增其RHD基因exon7与10,同时扩增SRY基因;另对exon 7、10和SRY都为阴性的标本检测甲基化RASSF1A基因作为胎儿DNA存在的标志。待胎儿分娩后,将基因检测结果与婴儿血清学检测结果比对,以评价该方法的准确性。结果 57位受检孕妇中,含RHD全部外显子者有17人;3人含exon 1和10,为RHD1-CE(2-9)-D10杂化基因;37人不含外显子。后两者40名孕妇中,22人检测出SRY基因,出生胎儿均为男性;另有2人为假阴性结果。39人检测出exon 7和10,其中38人基因型结果与胎儿出生后血清学结果相符,1例假阳性结果;1人未检测到SRY、exon 7和10的标本,检测到RASSF1A证明胎儿DNA存在,且胎儿出生后证实为RhD阴性女婴。结论建立了基于RASSFIA为标志的、符合中国人RHD基因特点的RhD阴性孕妇血浆游离DNA中胎儿RHD基因的检测程序,可用于临床无损性产前胎儿RhD血型预测。

管中窥豹:肺癌液态活检的现状与挑战

肺癌是中国最常见的恶性肿瘤之一,亟需新的诊断方法来检测肿瘤并监测治疗反应。液态活检作为一种非侵入性的肿瘤检测方法在肺癌的早筛诊断和治疗管理中展现出巨大的潜力。液态活检通过分析血液中的循环肿瘤细胞(CTCs)、细胞游离DNA(cfDNA)和循环肿瘤DNA(ctDNA),能够提供关于肿瘤的遗传信息,有利于肺癌早期诊断、病情监测以及疗效评估。相较于传统的组织活检,液态活检具有操作简便、风险低、可以反复进行以及能更全面反映肿瘤异质性等优点。该文回顾了液态活检在肺癌中的应用现状,探讨当前液态活检技术面临的挑战。旨在为肺癌的精准诊疗提供科学依据,推动液态活检技术在临床实践中的应用和发展。

循环游离DNA在多发性肌炎和皮肌炎中的作用

目的:研究循环游离DNA(cfDNA)在多发性肌炎(PM)和皮肌炎(DM)中的作用。方法:使用PicoGreen试剂盒检测61例PM/DM患者、34例系统性红斑狼疮(SLE)患者和48例健康对照的血浆cfDNA浓度,并与患者的血清学指标做相关性分析。结果:cfDNA浓度在PM/DM组是247.1±61.09ng/ml,显著高于健康对照组(197.1±31.36ng/ml,P<0.01),显著低于SLE组(281.9±82.21ng/ml,P<0.01)。cfDNA与血沉和血清球蛋白呈显著正相关(P<0.01,P<0.05),与C3呈显著负相关(P<0.01)。结论:cfDNA可能与PM/DM疾病活动度相关。

循环游离DNA的定量检测及面临的问题

循环游离DNA(circulating cell free DNA,cfDNA)与人类疾病之间存在着密切联系。近年来,cfDNA做为一种无创检测生物标志物,展现出临床应用前景。人们针对其含量较低的特点,进行了大量研究,开发出了各种较为可靠的定量检测方法。但目前cfDNA的定量检测仍然面临问题及争议,缺乏规范和标准化的流程。本文对cfDNA的来源组成、定量检测及存在的问题进行了归纳整理及分析,希望能对提高cfDNA的定量检测的可靠性提供有益的参考。