Robust and cost-effective CRISPR/Cas9 gene editing of primary tumor B cells in Eµ-TCL1 model of chronic lymphocytic leukemia

IF 7.6 2区 医学 Q1 HEMATOLOGY HemaSphere Pub Date : 2024-08-15 DOI:10.1002/hem3.134
Rosita Del Prete, Roberta Drago, Federica Nardi, Gaia Bartolini, Erika Bellini, Antonella De Rosa, Silvia Valensin, Anna Kabanova
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Gene editing via RNP electroporation has been recently applied to primary tumor cells isolated from patients chronic lymphocytic leukemia (CLL), suggesting an efficient and valuable tool for studying leukemic cell biology and biomarker validation.<span><sup>1, 2</sup></span> The work by Nardi et al. on this topic proposed to electroporate unmanipulated primary CLL cells that are subsequently put in culture with human CD40L-expressing fibroblasts and soluble stimuli to promote CLL cell proliferation. In this context, cellular proliferation is required to achieve homozygous gene editing, whereas in unstimulated CLL cells it is possible to achieve only the heterozygous editing.<span><sup>1</sup></span> The method published by Mateos-Jaimez et al. relies on the preactivation of CLL cells with CD40L/BAFF/IL-21-expressing stromal cells, followed by RNP electroporation and continuation of the stimulatory coculture.<span><sup>2</sup></span> Both methods approach 80%–90% of editing efficiency and allow to perform downstream <i>in vitro</i> experiments on edited leukemic cells.</p><p>Application of a similar RNP-based editing approach to the widely used murine model of CLL, the Eμ-TCL1 transgenic mice,<span><sup>3</sup></span> represents a valuable and versatile tool to explore CLL biology <i>in vivo</i>. Examples illustrating its feasibility has been first shown in studies by Chakraborthy et al. and Martines et al.<span><sup>4, 5</sup></span> The published method consists in preactivating primary CD19<sup>+</sup>CD5<sup>+</sup> leukemic B cells by TLR9 agonist CpG ODN-1668, followed by RNP electroporation and intraperitoneal injection of 30 × 10<sup>6</sup> electroporated cells to promote expansion of edited leukemic cells <i>in vivo</i>. Despite this method has been proven effective, it has not been set up to expand edited TCL1 cells <i>in vitro</i>. This is associated with high experimental costs and does not allow to perform functional analysis of gene editing phenotype prior to the <i>in vivo</i> transfer, which eventually becomes not feasible if edited cells are unfit <i>in vivo</i>.</p><p>Hence, we envisioned a new approach that would allow to expand RNP-electroporated TCL1 cells <i>in vitro</i> prior to transfer. To this end, we first optimized culture conditions for TCL1 cells evaluating their viability and proliferation after treatment with different stimuli. We observed that ODN-1668 stimulation, although being efficient in activating TCL1 cells in the short-term,<span><sup>5</sup></span> does not allow to expand them <i>in vitro</i> (Supporting Information S1: Figure S1). We thus evaluated different stimulation conditions and established that coculture of TCL1 cells with irradiated fibroblasts expressing murine CD40L was sufficient to induce proliferation of leukemic cells over 5 days of culture (Figure 1A,B). Curiously, IL-4 and IL-21 addition did not enhance CD40-driven TCL1 cell growth, in contrast to what is typically observed for human CLL cells (Figure 1A).</p><p>Next, we optimized electroporation settings for TCL1 cells using an <i>in vitro</i> translated mRNA encoding GFP<span><sup>1</sup></span> and an electroporation system with bimodal pulsing strategy previously employed by us for human CLL cell electroporation.<span><sup>1</sup></span> Among 13 tested electroporation conditions, the optimal one allowed us to maintain &gt;90% vitality of recovered TCL1 cells and achieve around 80% cell transfection efficiency (Figure 1C; electroporation settings in Supporting Information S1: Table S1; gating strategy in Supporting Information S1: Figure S2). To set up a protocol for CRISPR/Cas9 gene editing of TCL1 cells, we followed a pipeline indicated in Figure 1D. Electroporating TCL1 cells with polyglutamic acid-stabilized RNPs<span><sup>7</sup></span> and allowing them to proliferate 4–5 days post-electroporation typically allowed us to achieve &gt;80% gene KO in bulk population, either with single (Figure 1E,F) or double combination of sgRNAs (Figure 1G,H and Supporting Information S1: Figure S3). For example, targeting the surface marker CD19 proved convenient as a control that could be easily assessed by flow cytometry (Figure 1G,H). The protocol typically allowed for three-fold expansion of electroporated TCL1 cells, while maximum levels of gene silencing could be achieved by Day 4 of culturing (Figure S4). To expand Cas9/sgRNA-electroporated TCL1 cells <i>in vivo</i>, we used intravenous (<i>i.v.</i>) route of tumor infection into healthy C57BL/6 recipients<span><sup>8</sup></span> allowing for homogeneous tumor engraftment in C57BL/6 recipients at a reduced dose (5 × 10<sup>6</sup> cells per animal; Supporting Information S1: Figure S5).</p><p>In order to apply the newly developed protocol (Supporting Information Methods) to validate a relevant biomarker implicated in CLL pathogenesis, we decided to target the costimulatory receptor CD40, the triggering of which is sufficient to induce TCL1 cell proliferation (Figure 1A). CD40 engagement within CLL proliferative centers is thought to dictate CLL progression <i>in vivo</i><span><sup>9</sup></span> and promote resistance to therapies such as the Bcl2 inhibitor venetoclax.<span><sup>10</sup></span> We established sgRNA combination that was highly efficient in <i>Cd40</i> silencing <i>in vitro</i>, while silencing <i>Cd4</i> which is not expected to give any phenotype in TCL1 cells as a control (Figure 2A,B). Contrary to what expected, we observed that <i>Cd40</i> silencing did not affect CD40-driven TCL1 cell proliferation <i>in vitro</i>, suggesting that initial levels of CD40 protein might be sufficient to prime cells for proliferation and that at later time points CD40 signaling becomes dispensable (Figure 2C). We then performed an <i>in vivo</i> competition experiment by injecting <i>Cd40</i>-edited and <i>Cd4</i>-edited TCL1 cells into C57BL/6 recipients (Figure 2D). Resulting tumors maintained constant levels of <i>Cd40</i>-silenced tumor population that persisted <i>in vivo</i>, which was reflected in the constant frequency of <i>Cd40</i> locus indels in bulk tumor population (Figure 2D, right panel) and in a significantly lower CD40 expression compared to control tumors originating from <i>Cd4</i>-edited cells (Figure 2E,F). Our findings hence suggested that the loss of CD40 expression did not compromise expansion of leukemic cells <i>in vivo</i>. This result goes in line with a recently published observation that wild-type TCL1 cells are able to expand in CD40L<sup>−/−</sup> hosts.<span><sup>11</sup></span> Hence, complementary approaches allowing to test gene function in leukemia progression both by disrupting its expression on tumor cells, or within tumor microenvironment,<span><sup>11</sup></span> confidently illustrates that CD40 function may be substituted by other proliferative stimuli within CLL niche <i>in vivo</i>.</p><p>Our work reports a highly efficient and easily controlled genetic modification protocol for primary leukemic B cells in the TCL1 model. The whole cycle of gene silencing could be completed within 6–8 weeks from the start of sgRNA validation step, allowing to rapidly evaluate gene function in CLL progression. Our protocol routinely achieves over 80% editing efficiency and allows for quality control of CRISPR/Cas9 editing and functional assessment of gene silencing already in the <i>in vitro</i> phase. It lowers the cost of editing experiments as the <i>in vitro</i> TCL1 cell expansion allows for up to three-fold multiplication of edited cell population and proves effective in engrafting as low as 5 × 10<sup>6</sup> of edited TCL1 cells per animal via <i>i.v.</i> administration. Finally, our method is applicable to multiplexed gene editing <i>in vitro</i> and <i>in vivo</i> (Supporting Information S1: Figure S6) and could be translated to precise genome editing, wherein Cas9 RNPs are co-electroporated with a DNA template for homology-directed repair,<span><sup>12-15</sup></span> and to other B cell types, after appropriate set up of electroporation and expansion conditions.</p><p>Rosita Del Prete and Roberta Drago conceived the experimental design, performed experiments, analysed data and wrote the manuscript; Rosita Del Prete, Roberta Drago, Federica Nardi, Gaia Bartolini, Erika Bellini, Antonella De Rosa, and Silvia Valensin performed and analyzed experiments; Anna Kabanova coordinated the project, supervised experimental design, consulted obtained results, edited the manuscript and provided funding.</p><p>The authors declare no conflict of interest.</p>","PeriodicalId":12982,"journal":{"name":"HemaSphere","volume":"8 8","pages":""},"PeriodicalIF":7.6000,"publicationDate":"2024-08-15","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://onlinelibrary.wiley.com/doi/epdf/10.1002/hem3.134","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"HemaSphere","FirstCategoryId":"3","ListUrlMain":"https://onlinelibrary.wiley.com/doi/10.1002/hem3.134","RegionNum":2,"RegionCategory":"医学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"HEMATOLOGY","Score":null,"Total":0}
引用次数: 0

Abstract

Ability to genetically edit primary B cells via CRISPR/Cas9 technology represents a powerful tool to study molecular mechanisms of B-cell pathogenesis. In this context, employing ribonucleoprotein complexes (RNPs), formed by recombinant Cas9 and genome-targetting single guide RNA molecules, brings in advantage of accelerated set-up and protocol robustness. Gene editing via RNP electroporation has been recently applied to primary tumor cells isolated from patients chronic lymphocytic leukemia (CLL), suggesting an efficient and valuable tool for studying leukemic cell biology and biomarker validation.1, 2 The work by Nardi et al. on this topic proposed to electroporate unmanipulated primary CLL cells that are subsequently put in culture with human CD40L-expressing fibroblasts and soluble stimuli to promote CLL cell proliferation. In this context, cellular proliferation is required to achieve homozygous gene editing, whereas in unstimulated CLL cells it is possible to achieve only the heterozygous editing.1 The method published by Mateos-Jaimez et al. relies on the preactivation of CLL cells with CD40L/BAFF/IL-21-expressing stromal cells, followed by RNP electroporation and continuation of the stimulatory coculture.2 Both methods approach 80%–90% of editing efficiency and allow to perform downstream in vitro experiments on edited leukemic cells.

Application of a similar RNP-based editing approach to the widely used murine model of CLL, the Eμ-TCL1 transgenic mice,3 represents a valuable and versatile tool to explore CLL biology in vivo. Examples illustrating its feasibility has been first shown in studies by Chakraborthy et al. and Martines et al.4, 5 The published method consists in preactivating primary CD19+CD5+ leukemic B cells by TLR9 agonist CpG ODN-1668, followed by RNP electroporation and intraperitoneal injection of 30 × 106 electroporated cells to promote expansion of edited leukemic cells in vivo. Despite this method has been proven effective, it has not been set up to expand edited TCL1 cells in vitro. This is associated with high experimental costs and does not allow to perform functional analysis of gene editing phenotype prior to the in vivo transfer, which eventually becomes not feasible if edited cells are unfit in vivo.

Hence, we envisioned a new approach that would allow to expand RNP-electroporated TCL1 cells in vitro prior to transfer. To this end, we first optimized culture conditions for TCL1 cells evaluating their viability and proliferation after treatment with different stimuli. We observed that ODN-1668 stimulation, although being efficient in activating TCL1 cells in the short-term,5 does not allow to expand them in vitro (Supporting Information S1: Figure S1). We thus evaluated different stimulation conditions and established that coculture of TCL1 cells with irradiated fibroblasts expressing murine CD40L was sufficient to induce proliferation of leukemic cells over 5 days of culture (Figure 1A,B). Curiously, IL-4 and IL-21 addition did not enhance CD40-driven TCL1 cell growth, in contrast to what is typically observed for human CLL cells (Figure 1A).

Next, we optimized electroporation settings for TCL1 cells using an in vitro translated mRNA encoding GFP1 and an electroporation system with bimodal pulsing strategy previously employed by us for human CLL cell electroporation.1 Among 13 tested electroporation conditions, the optimal one allowed us to maintain >90% vitality of recovered TCL1 cells and achieve around 80% cell transfection efficiency (Figure 1C; electroporation settings in Supporting Information S1: Table S1; gating strategy in Supporting Information S1: Figure S2). To set up a protocol for CRISPR/Cas9 gene editing of TCL1 cells, we followed a pipeline indicated in Figure 1D. Electroporating TCL1 cells with polyglutamic acid-stabilized RNPs7 and allowing them to proliferate 4–5 days post-electroporation typically allowed us to achieve >80% gene KO in bulk population, either with single (Figure 1E,F) or double combination of sgRNAs (Figure 1G,H and Supporting Information S1: Figure S3). For example, targeting the surface marker CD19 proved convenient as a control that could be easily assessed by flow cytometry (Figure 1G,H). The protocol typically allowed for three-fold expansion of electroporated TCL1 cells, while maximum levels of gene silencing could be achieved by Day 4 of culturing (Figure S4). To expand Cas9/sgRNA-electroporated TCL1 cells in vivo, we used intravenous (i.v.) route of tumor infection into healthy C57BL/6 recipients8 allowing for homogeneous tumor engraftment in C57BL/6 recipients at a reduced dose (5 × 106 cells per animal; Supporting Information S1: Figure S5).

In order to apply the newly developed protocol (Supporting Information Methods) to validate a relevant biomarker implicated in CLL pathogenesis, we decided to target the costimulatory receptor CD40, the triggering of which is sufficient to induce TCL1 cell proliferation (Figure 1A). CD40 engagement within CLL proliferative centers is thought to dictate CLL progression in vivo9 and promote resistance to therapies such as the Bcl2 inhibitor venetoclax.10 We established sgRNA combination that was highly efficient in Cd40 silencing in vitro, while silencing Cd4 which is not expected to give any phenotype in TCL1 cells as a control (Figure 2A,B). Contrary to what expected, we observed that Cd40 silencing did not affect CD40-driven TCL1 cell proliferation in vitro, suggesting that initial levels of CD40 protein might be sufficient to prime cells for proliferation and that at later time points CD40 signaling becomes dispensable (Figure 2C). We then performed an in vivo competition experiment by injecting Cd40-edited and Cd4-edited TCL1 cells into C57BL/6 recipients (Figure 2D). Resulting tumors maintained constant levels of Cd40-silenced tumor population that persisted in vivo, which was reflected in the constant frequency of Cd40 locus indels in bulk tumor population (Figure 2D, right panel) and in a significantly lower CD40 expression compared to control tumors originating from Cd4-edited cells (Figure 2E,F). Our findings hence suggested that the loss of CD40 expression did not compromise expansion of leukemic cells in vivo. This result goes in line with a recently published observation that wild-type TCL1 cells are able to expand in CD40L−/− hosts.11 Hence, complementary approaches allowing to test gene function in leukemia progression both by disrupting its expression on tumor cells, or within tumor microenvironment,11 confidently illustrates that CD40 function may be substituted by other proliferative stimuli within CLL niche in vivo.

Our work reports a highly efficient and easily controlled genetic modification protocol for primary leukemic B cells in the TCL1 model. The whole cycle of gene silencing could be completed within 6–8 weeks from the start of sgRNA validation step, allowing to rapidly evaluate gene function in CLL progression. Our protocol routinely achieves over 80% editing efficiency and allows for quality control of CRISPR/Cas9 editing and functional assessment of gene silencing already in the in vitro phase. It lowers the cost of editing experiments as the in vitro TCL1 cell expansion allows for up to three-fold multiplication of edited cell population and proves effective in engrafting as low as 5 × 106 of edited TCL1 cells per animal via i.v. administration. Finally, our method is applicable to multiplexed gene editing in vitro and in vivo (Supporting Information S1: Figure S6) and could be translated to precise genome editing, wherein Cas9 RNPs are co-electroporated with a DNA template for homology-directed repair,12-15 and to other B cell types, after appropriate set up of electroporation and expansion conditions.

Rosita Del Prete and Roberta Drago conceived the experimental design, performed experiments, analysed data and wrote the manuscript; Rosita Del Prete, Roberta Drago, Federica Nardi, Gaia Bartolini, Erika Bellini, Antonella De Rosa, and Silvia Valensin performed and analyzed experiments; Anna Kabanova coordinated the project, supervised experimental design, consulted obtained results, edited the manuscript and provided funding.

The authors declare no conflict of interest.

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在 Eµ-TCL1 慢性淋巴细胞白血病模型中对原发肿瘤 B 细胞进行可靠且经济高效的 CRISPR/Cas9 基因编辑
CD40 在 CLL 增殖中心的参与被认为决定了 CLL 在体内的进展9 ,并促进对 Bcl2 抑制剂 venetoclax 等疗法的耐药性10 。我们建立了 sgRNA 组合,在体外对 Cd40 进行高效沉默,同时沉默 TCL1 细胞中预计不会产生任何表型的 Cd4 作为对照(图 2A、B)。与预期相反,我们观察到 Cd40 沉默并不影响体外 CD40 驱动的 TCL1 细胞增殖,这表明最初水平的 CD40 蛋白可能足以为细胞增殖提供能量,而在较晚的时间点,CD40 信号转导变得可有可无(图 2C)。然后,我们进行了体内竞争实验,将 Cd40 编辑和 Cd4 编辑的 TCL1 细胞注射到 C57BL/6 受体中(图 2D)。结果发现,体内Cd40沉默的肿瘤群体保持恒定水平,这反映在肿瘤群体中Cd40基因位点嵌合的恒定频率上(图2D,右图),以及与Cd4编辑细胞产生的对照肿瘤相比,CD40表达显著降低(图2E,F)。因此,我们的研究结果表明,CD40表达的缺失并不会影响白血病细胞在体内的扩增。这一结果与最近发表的一项观察结果一致,即野生型 TCL1 细胞能够在 CD40L-/- 宿主体内扩增。11 因此,通过破坏基因在肿瘤细胞或肿瘤微环境中的表达来测试基因在白血病进展中的功能的互补方法,11 有力地说明了 CD40 的功能可能会被体内 CLL 龛内的其他增殖刺激物所替代。从 sgRNA 验证步骤开始,整个基因沉默周期可在 6-8 周内完成,从而可快速评估基因在 CLL 进展中的功能。我们的方案通常能达到 80% 以上的编辑效率,并能在体外阶段对 CRISPR/Cas9 编辑进行质量控制和基因沉默的功能评估。它降低了编辑实验的成本,因为体外 TCL1 细胞扩增可使编辑过的细胞数量增加三倍,并证明通过静脉注射每只动物可有效移植低至 5 × 106 个编辑过的 TCL1 细胞。最后,我们的方法适用于体外和体内的多重基因编辑(佐证资料 S1:图 S6),在适当设置电穿孔和扩增条件后,可转化为精确的基因组编辑(Cas9 RNPs 与 DNA 模板共同电穿孔,用于同源定向修复)12-15 和其他 B 细胞类型。罗西塔-德尔普雷特(Rosita Del Prete)和罗贝塔-德拉戈(Roberta Drago)构思实验设计、进行实验、分析数据并撰写手稿;罗西塔-德尔普雷特、罗贝塔-德拉戈、费德里卡-纳尔迪、盖娅-巴托里尼、埃里卡-贝里尼、安东内拉-德罗莎和西尔维娅-瓦伦辛进行实验并分析数据;安娜-卡巴诺娃(Anna Kabanova)协调项目、指导实验设计、对获得的结果进行咨询、编辑手稿并提供资金。
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来源期刊
HemaSphere
HemaSphere Medicine-Hematology
CiteScore
6.10
自引率
4.50%
发文量
2776
审稿时长
7 weeks
期刊介绍: HemaSphere, as a publication, is dedicated to disseminating the outcomes of profoundly pertinent basic, translational, and clinical research endeavors within the field of hematology. The journal actively seeks robust studies that unveil novel discoveries with significant ramifications for hematology. In addition to original research, HemaSphere features review articles and guideline articles that furnish lucid synopses and discussions of emerging developments, along with recommendations for patient care. Positioned as the foremost resource in hematology, HemaSphere augments its offerings with specialized sections like HemaTopics and HemaPolicy. These segments engender insightful dialogues covering a spectrum of hematology-related topics, including digestible summaries of pivotal articles, updates on new therapies, deliberations on European policy matters, and other noteworthy news items within the field. Steering the course of HemaSphere are Editor in Chief Jan Cools and Deputy Editor in Chief Claire Harrison, alongside the guidance of an esteemed Editorial Board comprising international luminaries in both research and clinical realms, each representing diverse areas of hematologic expertise.
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