Next-generation sequencing and high DNA input identify previously missed measurable residual disease in peripheral blood of B-cell precursor acute lymphoblastic leukaemia

IF 5.1 2区医学 Q1 HEMATOLOGY

British Journal of Haematology Pub Date : 2024-10-24 DOI:10.1111/bjh.19834

Sonja Bendig, Sandra Bufe, Michaela Kotrova, Birgit Fricke, Constantin Proske, Franziska Darzentas, Nikos Darzentas, Anke Schilhabel, Britta Kehden, Guranda Chitadze, Claudia D. Baldus, Nicola Gökbuget, Monika Brüggemann

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Baldus, Nicola Gökbuget, Monika Brüggemann","doi":"10.1111/bjh.19834","DOIUrl":null,"url":null,"abstract":"In acute lymphoblastic leukaemia (ALL), measurable residual disease (MRD) is the most important prognostic factor for relapse.1, 2 Traditionally, MRD is quantified in bone marrow (BM) aspirates using real-time quantitative polymerase chain reaction (RQ-PCR) according to EuroMRD standards.3 The emergence of modern molecular methods has opened the possibility of MRD assessment from peripheral blood (PB), which causes less discomfort to patients and can therefore be performed more frequently, allowing a close monitoring of MRD levels. Furthermore, MRD assessment from PB could bypass technical challenges of BM aspiration, such as skewed or non-representative MRD values due to haemodilution and heterogenous distribution of leukaemic cells in different body compartments.4, 5 However, while comparable MRD values of BM and PB are observed for T-ALL,6, 7 in B-cell precursor ALL (BCP-ALL), MRD determination from PB is still a challenge. In both paediatric and adult cases, mean MRD levels in PB are consistently significantly lower compared to BM and frequently escape detection.6, 7 Additionally, paired samples exhibit a marked variability in the MRD level ratio.6Nevertheless, BCP-ALL patients with MRD positivity in the BM likely also harbour circulating leukaemic cells, even when missed by traditional methods. The implementation of more sensitive assays may enhance MRD detection from PB in these cases. To target this question, we retrospectively selected paired BM-PB samples of patients with BCP-ALL and BM MRD positivity where conventional RQ-PCR of clonal immunoglobulin heavy chain (IGH) VJ complete/DJ incomplete gene rearrangements did not detect PB MRD and reanalysed them with heightened sensitivity by using increased DNA input and amplicon-based next-generation sequencing (NGS).In total, 69 patients with pre/c-B-ALL (n = 57) or pro-B-ALL (n = 12) treated according to protocols of the German Multicentre Study Group on Adult ALL (GMALL) were included. All patients provided written informed consent for storage and use of the leftover material for medical research purposes. The Ethics Committee of the Medical Faculty at Christian-Albrechts-University of Kiel approved that there are no ethical or legal concerns about the conduct of the study (reference number D-402/21). Patient age ranged from 19 to 72 years with a median of 44 years. Of the analysed sample pairs, 52 were taken in first-line therapy and 17 during salvage treatment. IGH MRD markers were identified in the diagnostic samples using the EuroClonality amplicon-based NGS assay8 and the respective interpretation guidelines leading to a total of 80 IGH RQ-PCR assays (mean of 1.2 IGH assays/patient). RQ-PCR-based MRD quantification as part of the GMALL reference diagnostics was performed by standard RQ-PCR with 1.5 μg DNA in BM and PB, respectively, according to EuroMRD guidelines.3 In cases where more than one MRD marker was used per patient, the highest measured value was considered the cumulative MRD value. In all included cases, BM was MRD positive (41 with quantifiable MRD positivity and 28 with positivity below quantitative range) and PB was MRD negative using standard RQ-PCR with a sensitivity of at least 10−4. BM samples with a non-quantifiable MRD positivity were only included if subsequent BM samples were positive within the quantifiable range.For MRD re-evaluation, PB samples were reanalysed using the following approaches: (1) For high DNA input RQ-PCR, a total 6.6 μg DNA (corresponding to the DNA content of one million cells) was used and analysed in 10 separate reactions. (2) Amplicon-based NGS was performed with standard DNA input using 1.5 μg DNA, as well as with (3) high DNA input using 6.6 μg DNA in four different reactions. NGS MRD analyses were performed with the EuroClonality amplicon-based NGS assays.8 A 100-fold coverage of the spike-in rearrangements in the respective library or a minimum read amount of 300 000 was reached for all samples. Identification and quantification of leukaemia-derived clonotypes were done using ARResT/Interrogate.9, 10 In the NGS analyses, MRD values were termed not quantifiable when the percentage of positive marker reads corresponded to less than one cell equivalent (4 × 10−6 for standard input NGS, 10−6 for high input NGS).To assess the effect of high DNA input alone (approach 1), RQ-PCR from PB was performed for 57 of the 69 patients, for which sufficient leftover DNA was available. With this approach, at least one positive PCR signal was detected in 18/57 patients (32%; Figure 1A,B). None of the cases qualified as quantifiable MRD positive according to EuroMRD guidelines, which would require all 10 replicates to produce a positive signal within the specificity range.To assess the effect of NGS, 69 PB samples were NGS tested with standard (approach 2) and high DNA input (approach 3). With standard DNA input, MRD was detected in 16/69 patients (23%) (Figure 1A). In the high DNA input approach, MRD was detected in 33/69 patients (48%) (Figure 1A,B). All quantifiable MRD values were below 10−4, and in each case lower than in the corresponding BM sample.In these direct comparisons, only those IGH VJ/DJ markers that were also used for RQ-PCR were tracked by NGS. However, an important advantage of NGS is the ability to monitor all potential markers of a respective rearrangement type. For 37 of the 69 patients (54%), at least one additional valid IGH VJ/DJ marker was detected at initial diagnosis, which had not been used for routine RQ-PCR. In total, a mean of 2.3 valid IGH markers per patient was identified by NGS at initial diagnosis, but only a mean of 1.2 IGH markers per patient was used for MRD assessment by RQ-PCR. Considering all possible IGH markers improved NGS MRD detection in PB (Figure 1A) and identified MRD in three additional PB samples using high DNA input (Figures 1A and 2). Overall, MRD from PB was detected in 36/69 patients (52%) using this approach.Monitoring all potential IGH markers with NGS, therefore, increases the chance of detecting MRD. Although the majority of IGH clonotypes detected in the follow-up, PB samples derived from highly abundant diagnostic IGH clonotypes (52% of MRD-positive IGH markers were present in more than 50% of the target reads in the diagnostic sample) and also the lower abundant clonotypes contributed to MRD detection in PB (11% of MRD-positive IGH markers were present in only 5–10% of the target reads at initial diagnosis; Figure S1).However, the strategy of tracing not only the most abundant IGH clonotypes but also IGH rearrangements with lower abundance must be applied with caution. Low abundant clonotypes may not represent the leukaemia but minor accompanying B-cell clones leading to incorrect MRD results. As a precaution in accordance with the EuroClonality NGS guidelines, only markers with an abundance of >5% reads should be used, which could be clearly assigned to the leukaemia in a validation study.8 Nevertheless, the presence of monoclonal B-cell lymphocytosis (MBL) clones in individual patients cannot be ruled out. The risk of monoclonal B-cell expansions increases with patient age, with MBL being reported in up to 10% of healthy adults aged 50–59 years.11 Therefore, before implementation of this strategy into clinical routine, strict criteria have to be established for which markers can be used for MRD assessment. This is currently done within the EuroMRD Consortium.It should be noted that the distinction between quantified and non-quantified MRD values also stems from the varying methods of quantification. While the guidelines for RQ-PCR evaluation have been standardized for years, there are still no established definitions for quantitative range or non-quantifiable positivity in NGS.Overall, our results indicate that PB can be valuable for early MRD detection in BCP-ALL when adjusting traditional MRD assessment strategies. Still, MRD values in PB were significantly lower compared to BM and NGS with high DNA input only allowed MRD detection in half of the investigated cases, although it is very likely that tumour cells circulate in virtually all BM MRD-positive patients. Potentially, the frequency of leukaemia cells in the blood in these cases is so low that the sample volume limits MRD detection, as the denominator of the detection limit is the number of cell equivalents tested. Even with adjusted methods, PB therefore cannot replace BM for MRD assessment in BCP-ALL yet and BM monitoring should be sustained at critical stages of treatment protocols and during long-term follow-up, as relying on PB monitoring alone could delay the detection of an early relapse. However, in cases where a BM sample is not available, high DNA input and NGS should be considered to enhance the assay sensitivity and, consequently, increase the probability of detecting low-level MRD in PB.MB, NG, AS and MK designed the study, MB, MK, BK and SBu collected and selected patient data. SBu, SBe and BF performed the experiments. MB, CDB, MK, SBu, SBe and GC interpreted the data. CD, FD, BK and ND performed the bioinformatic data analysis. NG provided patient information. SBe wrote the first draft of the manuscript. All authors approved the final version of the manuscript.CB is consulting Astellas, BMS, AstraZeneca, Amgen, Jazz Pharmaceuticals, Gilead and Jannsen. NG received research funding from Novartis and research funding/Honoria from Pfizer, Jazz Pharmaceuticals, Incyte, Clinigen, Servier, Gilead and Amgen and honoraria from Autolus. MB is a member of Incytes and Amgens Board of Directors or advisory committees and the Speakers Bureaus of BD, Janssen, Pfizer and Amgen and received research funding from Amgen, Affimed and Regeneron. 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引用次数: 0

Abstract

In acute lymphoblastic leukaemia (ALL), measurable residual disease (MRD) is the most important prognostic factor for relapse.^{1, 2} Traditionally, MRD is quantified in bone marrow (BM) aspirates using real-time quantitative polymerase chain reaction (RQ-PCR) according to EuroMRD standards.³ The emergence of modern molecular methods has opened the possibility of MRD assessment from peripheral blood (PB), which causes less discomfort to patients and can therefore be performed more frequently, allowing a close monitoring of MRD levels. Furthermore, MRD assessment from PB could bypass technical challenges of BM aspiration, such as skewed or non-representative MRD values due to haemodilution and heterogenous distribution of leukaemic cells in different body compartments.^{4, 5} However, while comparable MRD values of BM and PB are observed for T-ALL,^{6, 7} in B-cell precursor ALL (BCP-ALL), MRD determination from PB is still a challenge. In both paediatric and adult cases, mean MRD levels in PB are consistently significantly lower compared to BM and frequently escape detection.^{6, 7} Additionally, paired samples exhibit a marked variability in the MRD level ratio.⁶

Nevertheless, BCP-ALL patients with MRD positivity in the BM likely also harbour circulating leukaemic cells, even when missed by traditional methods. The implementation of more sensitive assays may enhance MRD detection from PB in these cases. To target this question, we retrospectively selected paired BM-PB samples of patients with BCP-ALL and BM MRD positivity where conventional RQ-PCR of clonal immunoglobulin heavy chain (IGH) VJ complete/DJ incomplete gene rearrangements did not detect PB MRD and reanalysed them with heightened sensitivity by using increased DNA input and amplicon-based next-generation sequencing (NGS).

In total, 69 patients with pre/c-B-ALL (n = 57) or pro-B-ALL (n = 12) treated according to protocols of the German Multicentre Study Group on Adult ALL (GMALL) were included. All patients provided written informed consent for storage and use of the leftover material for medical research purposes. The Ethics Committee of the Medical Faculty at Christian-Albrechts-University of Kiel approved that there are no ethical or legal concerns about the conduct of the study (reference number D-402/21). Patient age ranged from 19 to 72 years with a median of 44 years. Of the analysed sample pairs, 52 were taken in first-line therapy and 17 during salvage treatment. IGH MRD markers were identified in the diagnostic samples using the EuroClonality amplicon-based NGS assay⁸ and the respective interpretation guidelines leading to a total of 80 IGH RQ-PCR assays (mean of 1.2 IGH assays/patient). RQ-PCR-based MRD quantification as part of the GMALL reference diagnostics was performed by standard RQ-PCR with 1.5 μg DNA in BM and PB, respectively, according to EuroMRD guidelines.³ In cases where more than one MRD marker was used per patient, the highest measured value was considered the cumulative MRD value. In all included cases, BM was MRD positive (41 with quantifiable MRD positivity and 28 with positivity below quantitative range) and PB was MRD negative using standard RQ-PCR with a sensitivity of at least 10⁻⁴. BM samples with a non-quantifiable MRD positivity were only included if subsequent BM samples were positive within the quantifiable range.

For MRD re-evaluation, PB samples were reanalysed using the following approaches: (1) For high DNA input RQ-PCR, a total 6.6 μg DNA (corresponding to the DNA content of one million cells) was used and analysed in 10 separate reactions. (2) Amplicon-based NGS was performed with standard DNA input using 1.5 μg DNA, as well as with (3) high DNA input using 6.6 μg DNA in four different reactions. NGS MRD analyses were performed with the EuroClonality amplicon-based NGS assays.⁸ A 100-fold coverage of the spike-in rearrangements in the respective library or a minimum read amount of 300 000 was reached for all samples. Identification and quantification of leukaemia-derived clonotypes were done using ARResT/Interrogate.^{9, 10} In the NGS analyses, MRD values were termed not quantifiable when the percentage of positive marker reads corresponded to less than one cell equivalent (4 × 10⁻⁶ for standard input NGS, 10⁻⁶ for high input NGS).

To assess the effect of high DNA input alone (approach 1), RQ-PCR from PB was performed for 57 of the 69 patients, for which sufficient leftover DNA was available. With this approach, at least one positive PCR signal was detected in 18/57 patients (32%; Figure 1A,B). None of the cases qualified as quantifiable MRD positive according to EuroMRD guidelines, which would require all 10 replicates to produce a positive signal within the specificity range.

To assess the effect of NGS, 69 PB samples were NGS tested with standard (approach 2) and high DNA input (approach 3). With standard DNA input, MRD was detected in 16/69 patients (23%) (Figure 1A). In the high DNA input approach, MRD was detected in 33/69 patients (48%) (Figure 1A,B). All quantifiable MRD values were below 10⁻⁴, and in each case lower than in the corresponding BM sample.

In these direct comparisons, only those IGH VJ/DJ markers that were also used for RQ-PCR were tracked by NGS. However, an important advantage of NGS is the ability to monitor all potential markers of a respective rearrangement type. For 37 of the 69 patients (54%), at least one additional valid IGH VJ/DJ marker was detected at initial diagnosis, which had not been used for routine RQ-PCR. In total, a mean of 2.3 valid IGH markers per patient was identified by NGS at initial diagnosis, but only a mean of 1.2 IGH markers per patient was used for MRD assessment by RQ-PCR. Considering all possible IGH markers improved NGS MRD detection in PB (Figure 1A) and identified MRD in three additional PB samples using high DNA input (Figures 1A and 2). Overall, MRD from PB was detected in 36/69 patients (52%) using this approach.

Monitoring all potential IGH markers with NGS, therefore, increases the chance of detecting MRD. Although the majority of IGH clonotypes detected in the follow-up, PB samples derived from highly abundant diagnostic IGH clonotypes (52% of MRD-positive IGH markers were present in more than 50% of the target reads in the diagnostic sample) and also the lower abundant clonotypes contributed to MRD detection in PB (11% of MRD-positive IGH markers were present in only 5–10% of the target reads at initial diagnosis; Figure S1).

However, the strategy of tracing not only the most abundant IGH clonotypes but also IGH rearrangements with lower abundance must be applied with caution. Low abundant clonotypes may not represent the leukaemia but minor accompanying B-cell clones leading to incorrect MRD results. As a precaution in accordance with the EuroClonality NGS guidelines, only markers with an abundance of >5% reads should be used, which could be clearly assigned to the leukaemia in a validation study.⁸ Nevertheless, the presence of monoclonal B-cell lymphocytosis (MBL) clones in individual patients cannot be ruled out. The risk of monoclonal B-cell expansions increases with patient age, with MBL being reported in up to 10% of healthy adults aged 50–59 years.¹¹ Therefore, before implementation of this strategy into clinical routine, strict criteria have to be established for which markers can be used for MRD assessment. This is currently done within the EuroMRD Consortium.

It should be noted that the distinction between quantified and non-quantified MRD values also stems from the varying methods of quantification. While the guidelines for RQ-PCR evaluation have been standardized for years, there are still no established definitions for quantitative range or non-quantifiable positivity in NGS.

Overall, our results indicate that PB can be valuable for early MRD detection in BCP-ALL when adjusting traditional MRD assessment strategies. Still, MRD values in PB were significantly lower compared to BM and NGS with high DNA input only allowed MRD detection in half of the investigated cases, although it is very likely that tumour cells circulate in virtually all BM MRD-positive patients. Potentially, the frequency of leukaemia cells in the blood in these cases is so low that the sample volume limits MRD detection, as the denominator of the detection limit is the number of cell equivalents tested. Even with adjusted methods, PB therefore cannot replace BM for MRD assessment in BCP-ALL yet and BM monitoring should be sustained at critical stages of treatment protocols and during long-term follow-up, as relying on PB monitoring alone could delay the detection of an early relapse. However, in cases where a BM sample is not available, high DNA input and NGS should be considered to enhance the assay sensitivity and, consequently, increase the probability of detecting low-level MRD in PB.

MB, NG, AS and MK designed the study, MB, MK, BK and SBu collected and selected patient data. SBu, SBe and BF performed the experiments. MB, CDB, MK, SBu, SBe and GC interpreted the data. CD, FD, BK and ND performed the bioinformatic data analysis. NG provided patient information. SBe wrote the first draft of the manuscript. All authors approved the final version of the manuscript.

CB is consulting Astellas, BMS, AstraZeneca, Amgen, Jazz Pharmaceuticals, Gilead and Jannsen. NG received research funding from Novartis and research funding/Honoria from Pfizer, Jazz Pharmaceuticals, Incyte, Clinigen, Servier, Gilead and Amgen and honoraria from Autolus. MB is a member of Incytes and Amgens Board of Directors or advisory committees and the Speakers Bureaus of BD, Janssen, Pfizer and Amgen and received research funding from Amgen, Affimed and Regeneron. For the remaining authors, no relevant conflicts of interest were declared.

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下一代测序和高 DNA 输入在 B 细胞前体急性淋巴细胞白血病患者的外周血中发现了之前遗漏的可测量的残留疾病。

在急性淋巴细胞白血病（ALL）中，可测量的残留病（MRD）是最重要的复发预后因素。传统上，MRD是根据EuroMRD标准使用实时定量聚合酶链反应（RQ-PCR）在骨髓（BM）抽吸物中定量的现代分子方法的出现使得外周血（PB） MRD评估成为可能，这对患者造成的不适较少，因此可以更频繁地进行，从而可以密切监测MRD水平。此外，通过PB进行MRD评估可以绕过BM抽吸的技术挑战，例如由于血液稀释和白血病细胞在不同体室的异质分布而导致的MRD值偏斜或不具有代表性。然而，虽然在T-ALL、b细胞前体ALL （BCP-ALL）中观察到BM和PB的MRD值相当，但从PB中测定MRD仍然是一个挑战。在儿童和成人病例中，与BM相比，PB的平均MRD水平始终显著低于BM，并且经常逃避检测。6,7此外，配对样本在MRD水平比率中表现出显著的可变性。然而，骨髓MRD阳性的BCP-ALL患者可能也有循环白血病细胞，即使传统方法没有发现。在这些病例中，实施更敏感的检测方法可能会提高铅的MRD检测。为了解决这个问题，我们回顾性地选择了BCP-ALL和BM MRD阳性患者的配对BM-PB样本，其中克隆免疫球蛋白重链（IGH） VJ完整/DJ不完整基因重排的常规RQ-PCR无法检测到PB MRD，并通过增加DNA输入和基于扩增子的下一代测序（NGS）以更高的灵敏度对它们进行了重新分析。共纳入69例pre/c-B-ALL患者（n = 57）或pro-B-ALL患者（n = 12），均按照德国成人ALL （GMALL）多中心研究组的方案进行治疗。所有患者都提供了书面知情同意，以便为医学研究目的储存和使用剩余材料。基尔基督教-阿尔布雷希茨-大学医学院伦理委员会批准，进行这项研究不存在伦理或法律问题（参考编号D-402/21）。患者年龄19 ~ 72岁，中位44岁。在分析的样本对中，52例为一线治疗，17例为抢救治疗。使用基于EuroClonality扩增子的NGS分析在诊断样本中鉴定出IGH MRD标记8和相应的解释指南，总共进行了80次IGH RQ-PCR分析（平均1.2次/患者）。基于RQ-PCR的MRD定量作为GMALL参考诊断的一部分，采用标准RQ-PCR，分别在BM和PB中添加1.5 μg DNA，按照EuroMRD指南进行在每个患者使用多个MRD标记物的情况下，最高测量值被认为是累积MRD值。在所有纳入的病例中，BM为MRD阳性（41例可量化MRD阳性，28例低于定量范围的阳性），PB为MRD阴性，使用标准RQ-PCR，灵敏度至少为10−4。不可量化MRD阳性的BM样品只有在后续BM样品在可量化范围内呈阳性时才被纳入。对于MRD重评价，采用以下方法对PB样品进行重分析：(1)对于高DNA输入RQ-PCR，共使用6.6 μg DNA（相当于100万个细胞的DNA含量），分10个反应进行分析。(2)采用标准输入1.5 μg的DNA和高输入6.6 μg的DNA进行扩增子基NGS反应。NGS MRD分析采用基于EuroClonality扩增子的NGS检测在各自的文库中，峰值重排的覆盖率达到100倍，或者所有样本的最小读取量达到30万。使用ARResT/Interrogate进行白血病衍生克隆型的鉴定和定量。9,10在NGS分析中，当阳性标记读数的百分比对应于少于一个细胞当量时，MRD值被称为不可量化（标准输入NGS为4 × 10−6，高输入NGS为10−6）。为了评估单独高DNA输入的效果（方法1），对69例患者中的57例进行了PB RQ-PCR，这些患者有足够的剩余DNA可用。采用该方法，57例患者中有18例(32%；图1 a, B)。根据EuroMRD指南，没有病例符合可量化MRD阳性，这需要所有10个重复在特异性范围内产生阳性信号。为了评估NGS的效果，我们对69份PB样本进行了标准（方法2）和高DNA输入（方法3）的NGS检测。在标准DNA输入下，69名患者中有16名（23%）检测到MRD（图1A）。在高DNA输入方法中，33/69例患者（48%）检测到MRD（图1A，B）。所有可量化的MRD值均低于10−4，且均低于相应的BM样品。在这些直接比较中，只有那些也用于RQ-PCR的IGH VJ/DJ标记被NGS跟踪。然而，NGS的一个重要优势是能够监测各自重排类型的所有潜在标记。69例患者中有37例（54%）在初始诊断时检测到至少一个额外的有效IGH VJ/DJ标记物，该标记物未用于常规RQ-PCR。总的来说，NGS在初始诊断时平均每位患者鉴定出2.3个有效的IGH标记物，但RQ-PCR用于MRD评估的平均每位患者只有1.2个IGH标记物。考虑到所有可能的IGH标记提高了NGS在PB中的MRD检测（图1A），并在另外三个使用高DNA输入的PB样本中鉴定了MRD（图1A和2）。总体而言，使用这种方法，69例患者中有36例（52%）检测到了PB的MRD。因此，用NGS监测所有潜在的IGH标记物增加了检测MRD的机会。尽管在随访中检测到大多数IGH克隆型，但PB样本来源于高丰度的诊断性IGH克隆型（52%的MRD阳性IGH标记存在于诊断样本中超过50%的靶读中），而且在PB中也有低丰度的克隆型有助于MRD检测（11%的MRD阳性IGH标记仅存在于最初诊断时的5-10%的靶读中）；图S1)。然而，不仅要追踪最丰富的IGH克隆型，而且要追踪丰度较低的IGH重排，必须谨慎使用。低丰度的克隆型可能不代表白血病，但伴随的少量b细胞克隆导致不正确的MRD结果。作为一项预防措施，根据EuroClonality NGS指南，只应使用具有&gt；5% reads丰度的标记，这可以在验证研究中明确地分配给白血病然而，不能排除个体患者中存在单克隆b细胞淋巴细胞增多症（MBL）克隆。单克隆b细胞扩增的风险随着患者年龄的增长而增加，据报道，在50-59岁的健康成年人中，高达10%的人患有MBL因此，在将该策略实施到临床常规之前，必须建立严格的标准，以确定可用于MRD评估的标记物。这是目前在EuroMRD联盟内完成的。应该注意的是，量化和非量化MRD值之间的区别也源于不同的量化方法。虽然RQ-PCR评估指南已经标准化多年，但对于NGS的定量范围或不可量化的阳性仍然没有既定的定义。总之，我们的研究结果表明，在调整传统MRD评估策略时，PB对BCP-ALL的早期MRD检测有价值。尽管如此，与BM和高DNA输入的NGS相比，PB的MRD值明显较低，尽管在几乎所有BM MRD阳性患者中肿瘤细胞很可能循环，但仅在一半的调查病例中允许MRD检测。可能，在这些病例中，血液中白血病细胞的频率非常低，以至于样本量限制了MRD检测，因为检测限的分母是被检测的细胞当量的数量。因此，即使采用调整后的方法，PB仍不能取代BM评估BCP-ALL的MRD，在治疗方案的关键阶段和长期随访期间，应持续进行BM监测，因为仅依靠PB监测可能会延迟早期复发的发现。然而，在没有BM样本的情况下，应该考虑高DNA输入和NGS来提高测定灵敏度，从而增加在PB中检测低水平MRD的可能性。MB、NG、AS和MK设计研究，MB、MK、BK和SBu收集和选择患者资料。SBu、SBe和BF进行了实验。MB、CDB、MK、SBu、SBe和GC对数据进行解释。CD、FD、BK和ND进行生物信息学数据分析。NG提供患者信息。他写了手稿的初稿。所有作者都认可了手稿的最终版本。世邦银行正在咨询安斯泰来、BMS、阿斯利康、安进、爵士制药、吉利德和杨森。NG获得了诺华的研究资金，辉瑞、Jazz Pharmaceuticals、Incyte、Clinigen、施维雅、吉利德和安进的研究资金和Autolus的研究资金。他是incyte和Amgens董事会或咨询委员会的成员，也是BD、Janssen、Pfizer和Amgen的发言人局的成员，并获得了Amgen、affirmed和Regeneron的研究资助。其余作者未发现相关利益冲突。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

British Journal of Haematology 医学-血液学

CiteScore

8.60

自引率

4.60%

发文量

565

审稿时长

1 months

期刊介绍： The British Journal of Haematology publishes original research papers in clinical, laboratory and experimental haematology. The Journal also features annotations, reviews, short reports, images in haematology and Letters to the Editor.