In Vitro and In Vivo Models of CLL–T Cell Interactions: Implications for Drug Testing

Hoferkova, Eva; Kadakova, Sona; Mráz, Marek

doi:10.3390/cancers14133087

Cited by 4 publications

(6 citation statements)

References 150 publications

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“…CD4+ T cells increase STAT6 driven BCR signaling through release of IL4 ( 56 ) and in normal B cells, this has been shown to be via activation of the non-canonical NF-κB pathway ( 57 ). CD4+ T cell activation of the non-canonical NF-κB pathway in CLL is also through CD40L activation of CD40 ( 58 , 59 ) and, as a result, CD40L and IL4 are important components of laboratory-based co-culture systems which aim to mimic the tumor microenvironment ( 40 , 60 , 61 ).…”

Section: The Cll Microenvironmentmentioning

confidence: 99%

NF-kB and the CLL microenvironment

et al. 2023

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Chronic lymphocytic leukemia (CLL) is the most prevalent type of leukemia in the western world. Despite the positive clinical effects of new targeted therapies, CLL still remains an incurable and refractory disease and resistance to treatments are commonly encountered. The Nuclear Factor-Kappa B (NF-κB) transcription factor has been implicated in the pathology of CLL, with high levels of NF-κB associated with disease progression and drug resistance. This aberrant NF-κB activation can be caused by genetic mutations in the tumor cells and microenvironmental factors, which promote NF-κB signaling. Activation can be induced via two distinct pathways, the canonical and non-canonical pathway, which result in tumor cell proliferation, survival and drug resistance. Therefore, understanding how the CLL microenvironment drives NF-κB activation is important for deciphering how CLL cells evade treatment and may aid the development of novel targeting therapeutics. The CLL microenvironment is comprised of various cells, including nurse like cells, mesenchymal stromal cells, follicular dendritic cells and CD4+ T cells. By activating different receptors, including the B cell receptor and CD40, these cells cause overactivity of the canonical and non-canonical NF-κB pathways. Within this review, we will explore the different components of the CLL microenvironment that drive the NF-κB pathway, investigating how this knowledge is being translated in the development of new therapeutics.

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Section: The Cll Microenvironmentmentioning

confidence: 99%

NF-kB and the CLL microenvironment

et al. 2023

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“…CLL cell birth rates in lymph nodes are 0.5-3% per day, and newborn CLL cells can exit the lymph nodes to the peripheral blood [2,3]. Lymph node niche is believed to promote CLL proliferation via microenvironmental factors such as the CD40, Toll-like receptors (TLR), and B-cell receptor (BCR) activation [3,4]. Notably, BCR crosslinking in vitro is insufficient to induce CLL proliferation [5], suggesting other microenvironmental interactions are needed to (co)drive proliferation.…”

Section: Introductionmentioning

confidence: 99%

“…Notably, BCR crosslinking in vitro is insufficient to induce CLL proliferation [5], suggesting other microenvironmental interactions are needed to (co)drive proliferation. The prime candidates for pro-proliferative signals are CLL-CD4 + T-cell interactions, since in vitro CLL cells can be stimulated to proliferate by CLL-T-cell contact [4][5][6][7][8][9]. Furthermore, in immunodeficient mice, CLL cell engraftment depends on the co-transplantation of activated T-cells [10,11].…”

Section: Introductionmentioning

confidence: 99%

“…Studies of normal B-cells point to CD40 ligand's (CD40L/CD154) crucial relevance in normal B-cell proliferation and its synchronization with BCR activation in germinal centers [16]. In CLL, CD40 stimulation alone is not sufficient to drive proliferation and must be combined with other factors, such as adding recombinant IL4, IL21, or CpG-ODN [4,5,17]. This activates downstream signaling largely shared with BCR, including NFκB, AKT, MYC, and MAPK/ERK (reviewed in [18]).…”

Section: Introductionmentioning

confidence: 99%

“…Several in vitro microenvironment model systems have been developed to study CLL biology, perform in vitro screening of chemical libraries for compounds with anti-CLL activity, and guide therapeutic decisions [19][20][21][22]. Most such co-culture models involve human or murine fibroblast-like stromal cells that provide signals to overcome spontaneous CLL cell apoptosis and/or mimic adhesion-mediated drug resistance, but these do not trigger proliferation [4,[22][23][24][25]. To induce proliferation, co-culture models typically utilize costly recombinant factors like IL4 or IL21 added to co-cultures with CD40L-expressing stromal cells; however, in such conditions, the CLL proliferation rate is relatively low and highly variable [9,26].…”

Section: Introductionmentioning

confidence: 99%

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Stromal cells engineered to express T cell factors induce robust CLL cell proliferation in vitro and in PDX co-transplantations allowing the identification of RAF inhibitors as anti-proliferative drugs

Hoferkova,

Seda,

Kadakova

et al. 2024

Leukemia

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Several in vitro models have been developed to mimic chronic lymphocytic leukemia (CLL) proliferation in immune niches; however, they typically do not induce robust proliferation. We prepared a novel model based on mimicking T-cell signals in vitro and in patient-derived xenografts (PDXs). Six supportive cell lines were prepared by engineering HS5 stromal cells with stable expression of human CD40L, IL4, IL21, and their combinations. Co-culture with HS5 expressing CD40L and IL4 in combination led to mild CLL cell proliferation (median 7% at day 7), while the HS5 expressing CD40L, IL4, and IL21 led to unprecedented proliferation rate (median 44%). The co-cultures mimicked the gene expression fingerprint of lymph node CLL cells (MYC, NFκB, and E2F signatures) and revealed novel vulnerabilities in CLL-T-cell-induced proliferation. Drug testing in co-cultures revealed for the first time that pan-RAF inhibitors fully block CLL proliferation. The co-culture model can be downscaled to five microliter volume for large drug screening purposes or upscaled to CLL PDXs by HS5-CD40L-IL4 ± IL21 co-transplantation. Co-transplanting NSG mice with purified CLL cells and HS5-CD40L-IL4 or HS5-CD40L-IL4-IL21 cells on collagen-based scaffold led to 47% or 82% engraftment efficacy, respectively, with ~20% of PDXs being clonally related to CLL, potentially overcoming the need to co-transplant autologous T-cells in PDXs.

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