Dendritic and axonal morphology reflects the input and output of neurons and is a defining feature of neuronal types1,2, yet our knowledge of its diversity remains limited. Here, to systematically examine complete single-neuron morphologies on a brain-wide scale, we established a pipeline encompassing sparse labelling, whole-brain imaging, reconstruction, registration and analysis. We fully reconstructed 1,741 neurons from cortex, claustrum, thalamus, striatum and other brain regions in mice. We identified 11 major projection neuron types with distinct morphological features and corresponding transcriptomic identities. Extensive projectional diversity was found within each of these major types, on the basis of which some types were clustered into more refined subtypes. This diversity follows a set of generalizable principles that govern long-range axonal projections at different levels, including molecular correspondence, divergent or convergent projection, axon termination pattern, regional specificity, topography, and individual cell variability. Although clear concordance with transcriptomic profiles is evident at the level of major projection type, fine-grained morphological diversity often does not readily correlate with transcriptomic subtypes derived from unsupervised clustering, highlighting the need for single-cell cross-modality studies. Overall, our study demonstrates the crucial need for quantitative description of complete single-cell anatomy in cell-type classification, as single-cell morphological diversity reveals a plethora of ways in which different cell types and their individual members may contribute to the configuration and function of their respective circuits.
IPD patients have a higher prevalence of PN than controls. Although causality is not established, levodopa exposure is associated with MMA elevation and sensorimotor neuropathy in IPD patients. Cobalamin replacement concurrent with levodopa therapy should be considered to protect against development of PN in IPD patients.
To develop an ideal blood clot imaging and targeting agent, a single-chain antibody (SCA) fragment based on a fibrin-specific monoclonal antibody, MH-1, was constructed and produced via secretion from Bacillus subtilis. Through a systematic study involving a series of B. subtilis strains, insufficient intracellular and extracytoplasmic molecular chaperones and high sensitivity to wall-bound protease (WprA) were believed to be the major factors that lead to poor production of MH-1 SCA. Intracellular and extracytoplasmic molecular chaperones apparently act in a sequential manner. The combination of enhanced coproduction of both molecular chaperones and wprA inactivation leads to the development of an engineered B. subtilis strain, WB800HM[pEPP]. This strain allows secretory production of MH-1 SCA at a level of 10 to 15 mg/liter. In contrast, with WB700N (a seven-extracellular-protease-deficient strain) as the host, no MH-1 SCA could be detected in both secreted and cellular fractions. Secreted MH-1 SCA from WB800HM[pMH1, pEPP] could be affinity purified using a protein L matrix. It retains comparable affinity and specificity as the parental MH-1 monoclonal antibody. This expression system can potentially be applied to produce other single-chain antibody fragments, especially those with folding and protease sensitivity problems.
Since the downregulation of I(tof) was observed with overexpression of calcineurin and was also reversed by the calcineurin inhibitor CsA, we conclude that downregulation of I(tof) is a consequence of calcineurin overexpression.
32Ever since the seminal findings of Ramon y Cajal, dendritic and axonal morphology has been 33 recognized as a defining feature of neuronal types and their connectivity. Yet our knowledge 34 about the diversity of neuronal morphology, in particular its distant axonal projections, is still 35 extremely limited. To systematically obtain single neuron full morphology on a brain-wide scale 36in mice, we established a pipeline that encompasses five major components: sparse labeling, 37whole-brain imaging, reconstruction, registration, and classification. We achieved sparse, robust 38and consistent fluorescent labeling of a wide range of neuronal types across the mouse brain in 39 an efficient way by combining transgenic or viral Cre delivery with novel transgenic reporter 40 lines, and generated a large set of high-resolution whole-brain fluorescent imaging datasets 41containing thousands of reconstructable neurons using the fluorescence micro-optical sectioning 42 tomography (fMOST) system. We developed a set of software tools based on the visualization 43 and analysis suite, Vaa3D, for large-volume image data processing and computation-assisted 44 morphological reconstruction. In a proof-of-principle case, we reconstructed full morphologies 45 of 96 neurons from the claustrum and cortex that belong to a single transcriptomically-defined 46 neuronal subclass. We developed a data-driven clustering approach to classify them into multiple 47 morphological and projection types, suggesting that these neurons work in a targeted and 48coordinated manner to process cortical information. Imaging data and the new computational 49 reconstruction tools are publicly available to enable community-based efforts towards large-scale 50 full morphology reconstruction of neurons throughout the entire mouse brain. 51 52 53
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