Analysis of Marker-Defined HNSCC Subpopulations Reveals a Dynamic Regulation of Tumor Initiating Properties

Head and neck squamous carcinoma (HNSCC) tumors carry dismal long-term prognosis and the role of tumor initiating cells (TICs) in this cancer is unclear. We investigated in HNSCC xenografts whether specific tumor subpopulations contributed to tumor growth. We used a CFSE-based label retentions assay, CD49f (α6-integrin) surface levels and aldehyde dehydrogenase (ALDH) activity to profile HNSCC subpopulations. The tumorigenic potential of marker-positive and -negative subpopulations was tested in nude (Balb/c nu/nu) and NSG (NOD.Cg-Prkdcscid Il2rgtm1Wjl/SzJ) mice and chicken embryo chorioallantoic membrane (CAM) assays. Here we identified in HEp3, SQ20b and FaDu HNSCC xenografts a subpopulation of G0/G1-arrested slow-cycling CD49fhigh/ALDH1A1high/H3K4/K27me3low subpopulation (CD49f+) of tumor cells. A strikingly similar CD49fhigh/H3K27me3low subpopulation is also present in primary human HNSCC tumors and metastases. While only sorted CD49fhigh/ALDHhigh, label retaining cells (LRC) proliferated immediately in vivo, with time the CD49flow/ALDHlow, non-LRC (NLRC) tumor cell subpopulations were also able to regain tumorigenic capacity; this was linked to restoration of CD49fhigh/ALDHhigh, label retaining cells. In addition, CD49f is required for HEp3 cell tumorigenicity and to maintain low levels of H3K4/K27me3. CD49f+ cells also displayed reduced expression of the histone-lysine N-methyltransferase EZH2 and ERK1/2phosphorylation. This suggests that although transiently quiescent, their unique chromatin structure is poised for rapid transcriptional activation. CD49f− cells can “reprogram” and also achieve this state eventually. We propose that in HNSCC tumors, epigenetic mechanisms likely driven by CD49f signaling dynamically regulate HNSCC xenograft phenotypic heterogeneity. This allows multiple tumor cell subpopulations to drive tumor growth suggesting that their dynamic nature renders them a “moving target” and their eradication might require more persistent strategies

The nano-architecture of the axonal cytoskeleton

International audienceThe cytoskeleton is a cellular shapeshifter. Like these creatures of mythology and speculative fiction, the cytoskeleton can alter its physical form and shape to accommodate the immediate needs of the cell. Indeed, many a rapt student has watched the cytoskeleton of a dividing cell seemingly miraculously transform into an organized mitotic spindle and then dissolve into an indiscrete mass, right before their eyes. The extreme polarization of neurons (that is, their fundamental asymmetry, arising due to the presence of elongated processes), along with their lifelong plasticity, creates unique demands on the cytoskeleton. A remarkable example is the axon, which can grow to enormous lengths and must generate and maintain its form and function throughout life — a burden that rests largely on the cytoskeleton. The axonal cytoskeleton has three major constituents: microtubules, neurofilaments and actin (BOX 1). Each is unique, associating with its own set of binding proteins and performing specialized roles within the axon. Most of these cytoskeletal proteins are synthesized in the neu­ ronal soma and are transported along the axon. Such transport is a constitutive phenomenon that occurs throughout the life of the neuron. Thus, the axonal cytoskeleton is best understood by considering both its anatomical organization and its dynamics (including axonal transport). Given the complex morphology and physiology of neurons, the field of neurobiology has traditionally been at the forefront of adopting new optical techno­ logies as they arise. Advances in microscopy now allow us to observe cells with unprecedented spatial resolu­ tion and to follow dynamic processes with exquisite temporal detail 1. For example, super­resolution strat­ egies that circumvent the diffraction limit of optical microscopy appeared more than ten years ago (BOX 2) and have been used to reveal aspects of neuronal organ­ ization down to the scale of macromolecular com­ plexes 2. These techniques have provided key insights into the organization and function of the axonal cytoskeleton — and in particular the organization of actin and microtubules — revealing how it builds the axon and maintains its intricate architecture. Focusing on the cytoskeleton within the axon initial segment (AIS) and the more distal axon shaft, in this Review, we highlight these recent discoveries and place them in the context of earlier findings, giving the reader a tentative vision of the future. Overview of the axonal cytoskeleton The history of cytoskeletal research is essentially the pursuit of tools and techniques that allowed an ever­ closer view of this elaborate structure, a quest that continues to this day. Early studies by 17th­century microscopy pioneers highlighted a network of 'neu­ rofibrils' , which we now know were most likely neuro­ filaments 3. With the advent of electron microscopy, two types of fibrils were seen in axons: filaments measuring approximately 10 nm in diameter, corresponding to neurofilaments, and others measuring approximately 20–30 nm in diameter, corresponding to structures that eventually came to be known as microtubules 4,5. Abstract | The corporeal beauty of the neuronal cytoskeleton has captured the imagination of generations of scientists. One of the easiest cellular structures to visualize by light microscopy, its existence has been known for well over 100 years, yet we have only recently begun to fully appreciate its intricacy and diversity. Recent studies combining new probes with super-resolution microscopy and live imaging have revealed surprising details about the axonal cytoskeleton and, in particular, have discovered previously unknown actin-based structures. Along with traditional electron microscopy, these newer techniques offer a nanoscale view of the axonal cytoskeleton, which is important for our understanding of neuronal form and function, and lay the foundation for future studies. In this Review, we summarize existing concepts in the field and highlight contemporary discoveries that have fundamentally altered our perception of the axonal cytoskeleton