Monday, July 17, 2017

Electrical Preconditioning of Stem Cells

Cool Science

The ability to manipulate hNPCs via a conductive scaffold creates a new approach to optimize stem cell-based therapy and determine which factors (such as VEGF-A) are essential for stroke recovery: Paul M. Georgea, Tonya M. Blissb, Thuy Huab, Alex Leed, Byeongtaek Oh, Alexa Levinson, Swapnil Mehta, Guohua Sun, Gary K. Steinberg. Electrical preconditioning of stem cells with a conductive polymer scaffold enhances stroke recovery. doi.org/10.1016/j.biomaterials.2017.07.020...anti βIII-tubulin (1:500, Neuromics, Edina, MN)...

Image: Neural progenitors were labeled with anti-rat Nestin polyclonal antibody (Cat#:GT15114) and stained with conjugated donkey anti-goat secondary anti-body (green). Differentiated neurons were labeled with neuron-specific mouse anti-β-III tubulin/ Tuj1-(Cat#MO15013 monoclonal antibody (red). Nuclei were stained with DAPI (blue).
We have excellent Stem Cell Differentiation Markers. Check them out.

Tuesday, July 11, 2017

New Human RPES and BMSCS

Need Human Cells? Just Ask!

This is our cornerstone and we keep building on it. You asked for them. We are pleased to announce we now have Human Bone Marrow-Derived Stem Cells (BMSCs) and Retinal Pigment Epithelial Cells (RPES).
RPES in Culture.
BMSCS in Culture.
We will continue to post new cell offerings here.

Thursday, July 06, 2017

3D Printing the Way to Artificial Muscles

Muscles Contract Under the Control Motor Neurons

The methods used to develop the artificial muscles included use of our GDNF Protein to maintain motor neurons in the 3-D Culture-Caroline Cvetkovic, Max H. Rich, Ritu Raman, Hyunjoon Kong , Rashid Bashir. A 3D-printed platform for modular neuromuscular motor units. Microsystems; Nanoengineering 3, Article number: 17015 (2017) doi:10.1038/micronano.2017.15

Skeletal muscle cells and motor neurons were combined into a fabricated 3D co-culture system. C2C12 myoblasts were differentiated into multinucleated myotubes (a) and combined with extracellular matrix (ECM) proteins to create an engineered muscle ring tissue (b). In parallel, mouse embryonic stem cells (HBG3 mESCs) were differentiated into motor neurons (MNs) through the formation of embryoid bodies (EBs) (c and d) and then combined with the engineered muscle tissue and ECM proteins (e) on 3D-printed hydrogel devices (f and g). Once the multi-layered rings sequentially compacted and fused together, they were then placed on a stationary hydrogel skeleton (h). Scale bars, 50 μm (b and d), 500 μm (c), and 10 μm (d, inset).

Wednesday, July 05, 2017

Renal Nerves and Blood Pressure

Role of Calcitonin gene-related peptide (CGRP)

CGRP is a potent vasodilator so it is not surprising our CGRP Antibody was used in this study. Custódio AH, de Lima MC, Vaccari B, Boer PA, Gontijo JAR (2017) Renal sodium handling and blood pressure changes in gestational protein-restricted offspring: Role of renal nerves and ganglia neurokinin expression. PLoS ONE 12(6): e0179499. https://doi.org/10.1371/journal.pone.0179499

Figure. Comparative expression of SP and CGRP in the renal pelvis of 16-week-old rats. The pictures show a normal distribution of these neurokinins in NP (A and D). In LP offspring, no difference was observed in SP immunoreactivity (A, B, and C), but CGRP immunoreactivity was significantly more intense in NP (D, E, and F) compared with age-matched LP offspring.

We are always honored when our solutions are referenced in publications and will continue to post new findings here.

Tuesday, June 27, 2017

Petaka Cell Culturing System in Action

Used for Hypoxia Induction
Cells are the engine of cell-based assays. Our PetakaTM Cell Culture System knock-down barriers that stand between you and success. The system is especially designed to grow cells in an isolated, auto-modified environment, highly protected from external environmental conditions.

In this study, for hypoxia induction, Petaka G3 low oxygen transfer flasks (Neuromics) were used to culture melanoma cell lines or primary melanocytes for 48–96 h at 37°C until >80% confluent: Rachel L. G. Maus, James W. Jakub, Wendy K. Nevala, Trace A. Christensen, Klara Noble-Orcutt, Zohar Sachs, Tina J. Hieken, and Svetomir N. Markovic. Human Melanoma-Derived Extracellular Vesicles Regulate Dendritic Cell Maturation. Front Immunol. 2017; 8: 358. Published online 2017
Mar 29. doi: 10.3389/fimmu.2017.00358.

Hypoxia increases extracellular vesicles (EVs) production in metastatic melanoma cell line SKMEL28 not primary melanocytes. Melanoma cell lines and adult primary melanocytes were cultured under hypoxia or normoxia conditions for 48 h. Morphology and CD63 vesicle marker expression of SKMEL28 EVs was confirmed by immune electron microscopy (A) and vesicle size distribution and particle concentration measured by nanoparticle tracking analysis (Nanosight) [(B), representative image]. Total concentration of normoxic (gray) or hypoxic (black) vesicles isolated from three melanoma cell lines and healthy primary melanocytes was quantified by Nanosight following three replicate 30-s video captures of three EV preparations (C) (n = 3 independent experiments).

Petaka advantages include:

  • No requirement of CO2 incubator or humid incubator. 
  • Exact volume of media per culture. 
  • Cell growth on vertical walls segregates cells and debris. 
  • Negligible dehydration rates Protected against leaks or spills. 
  • Higher cell yields. 
  • Shipping and short term cell maintenance at room temperature.

Wednesday, June 21, 2017

Gap Junctions (GJs) and Glaucoma

GJs Can Offer Neuroprotection
This study references use of our GFAP Antibody,

Gap junctions (GJs), intercellular channels composed of subunit connexins, can play a major role in secondary cell death by forming conduits through which toxic molecules from dying cells pass to and injure coupled neighbors. Secondary cells like glia and astrocytes are involved in this process though the precise mechanisms have yet to be defined: Abram Akopian, Sandeep Kumar, Hariharasubramanian Ramakrishnan, Kaushambi Roy, Suresh Viswanathan, and Stewart A. Bloomfield. Targeting neuronal gap junctions in mouse retina offers neuroprotection in glaucoma. J Clin Invest. doi:10.1172/JCI91948. Copyright © 2017, The American Society for Clinical Investigation. ...anti-GFAP (1:1,000, RA22101; Neuromics)...

Figure: Reactive gliosis in retinas of microbead-injected mice is significantly reduced by GJ blockade/ablation. (A) Confocal images of retinal layers stained for GFAP, SMI32, and DAPI in control and glaucomatous retinas. Scale bar: 50 μm in all panels. Z-stack: 7 sections, 3-μm steps. (B) GFAP expression in the retinal layers of CxWT and Cx36–/– mouse retinas under different conditions (n = 6 retinas per group). (C) GFAP labeling in retinal sections from control and microbead-injected CxWT (n = 5 retinas), Cx36–/– (n = 5 retinas), and Cx36–/– Cx45–/– mice (n = 3 retinas). GFAP expression is presented as percentage of immunolabeling per area.
Our Neuron/Synapse, Astrocytes, Glia, Microglia, Oligodendrocytes, Progenitors and Schwann Cell Markers are frequently referenced and I will continue to post new developments.

Tuesday, June 13, 2017

Modeling HIV Latency

Generation of Infected Neurons
Researchers have developed a Neuronal Cell Line for the study of HSV-1 infection in humans. This line was developed by terminally differentiating human embryonic stem cells to neurons.

Our mouse monoclonal nestin antibody was used as a marker for the neural progenitor phase of this differentiation. Aldo Pourchet, Aram S. Modrek, Dimitris G. Placantonakis, Ian Mohr and Angus C. Wilson. Modeling HSV-1 Latency in Human Embryonic Stem Cell-Derived Neurons. Pathogens 2017, 6(2), 24; doi:10.3390/pathogens6020024.


Image:  In vitro derivation of human neural stem cells by differentiation of the Hes5::GFP human embryonic stem cell line. (A) Schematic showing the multistep neural induction protocol. TGFβi stands for TGF-β receptor I inhibitor (B) Bright field image of human embryonic stem cell (hESC) colonies cultured on mouse embryonic fibroblasts prior to reaching confluence. (C) Bright field image of rosette NSCs derived from dissociated hESC colonies cultured in neural induction media. (D) Phase contrast and indirect immunofluorescence images of NSC cultures grown on poly-l-ornithine/laminin-coated dishes in neural stem cell media and probed with an antibody against nestin, a neural stem cell marker. Nuclei were visualized with DAPI.
We will continue to post publications referencing use of our solutions.

Wednesday, June 07, 2017

Neuromics' Customers

How They Find Us and What they Buy

Trust is hard to maintain and easily lost. It is important to us that our customers can find us and the products required to meet their research needs.

In order to nurture trust, we follow up with each and every customer to make sure they are happy with their Neuromics' experience. We include the opportunity for them to formally rate this experience @ https://birdeye.com/neuromics-186498936.

We plan on rolling out a new website. Our goal is to make it even easier for customers to find us and present content in a way that aligns with customers' needs. This includes making sure content is configured in a way that works on all platforms used including mobile devices.

As part of the process, we recently surveyed users for areas of research, platforms used, how they find companies like ours and what the purchase. Here're rollups of some of the results.

Our customers most frequently purchase Antibodies and Markers. Cells and Cell-Based Assays are increasingly important, We plan on making it easier for users to find related protocols, publications, data and alternative product options.

Trust, for us, includes the ability for our customers to find the correct solutions and if they prove not to work, offer fixes or full refunds. As in the past, we will be posting updates, publications and customer generated data here.


Tuesday, June 06, 2017

New Website

Your Help Needed

We will be rolling out a new Neuromics' Website in August 2017. Our goal is to make it easy for you to find us and the solutions that meet your needs. Your input will help us achieve this. We have a short survey.

Tuesday, May 30, 2017

Rose Hip and Heart Disease

Helps Prevent Atherosclerotic Plaques

This study features the use of our ABCA1 Antibody. The ATP-binding cassette transporter (ABC) Protein called ABCA1 has a major impact on cellular and whole body cholesterol metabolism and is likely to play an important role in protecting against cardiovascular disease.

The authors conclude that rose hip is a suitable dietary supplement for preventing atherosclerotic plaques formation by modulating systemic blood pressure and the expression of RCT and inflammatory genes.Michele Cavalera, Ulrika Axling, Catarina Rippe, Karl Swärd, and Cecilia Holm. Dietary rose hip exerts anti-atherosclerotic effects and increases nitric oxide-mediated dilation in ApoE-null mice. The Journal of Nutritional Biochemistry. Available online 21 March 2017. http://dx.doi.org/10.1016/j.jnutbio.2017.02.017...Western blotting. Approximately 50 mg of tissue was homogenized in lysis buffer (50 mM Tris–HCl, pH 7.5, 1 mM EGTA, 1 mM EDTA, 1% NP40, 1 mM Na-orthovanadate, 40 mM NaF, 4 mM Na-pyrophosphate, 0.27 M sucrose, 1 mM DTT, 20 μg/ml leupeptin, 10 μg/ml antipain and 1 μg/ml pepstatin) and subsequently centrifuged at 12,000 g for 20 min at 4 °C. Protein concentration of the supernatant was determined using BCA-assay (Pierce) and 20 μg of proteins were resolved on NuPAGE 4–12% Bis-Tris Gel (Life Technologies – Carlsbad, CA) and electroblotted onto nitrocellulose membranes (Amersham, GE Healthcare – UK). The membranes were washed and incubated with primary and appropriate secondary antibodies. Primary antibodies used were: SR-B1 (ab3 - Abcam), beta-actin (A5441 – Sigma), Abca1 (MO13101 - Neuromics), Abcg1 (orb214917, Biorbyt), Abcg5 (orb5656, Biorbyt), Abcg8 (orb228808, Biorbyt), IL1b (orb101745, Biorbyt), IL6 (orb228222, Biorbyt), NF-kB (ab7970, Abcam) and HSP90 (BD610418, BD bioscience)...

RH supplementation modulates the reverse cholesterol transport pathway. (a) Liver qPCR analysis of cholesterol metabolism showed similar expression of genes involved in the synthesis and conversion of cholesterol into bile acids but increased expression of various RCT genes upon rose hip feeding (n=5–6).
(b) Protein levels of SR-B1, Abcg1 and Abcg5 were increased in the liver of RH-feeding mice (n=6). *P<.05, **P<.01 and ^P=.056 versus CTR.



We have an extensive catalog of Characterized, Tested and Research Ready Antibodies/Markers. Check us out.

Wednesday, May 24, 2017

Parkinson's Disease and the Striatum

Excellent Video
Researchers at the Karolinska Institute recently released a video outlining their findings regarding the root causes of Parkinson's.


Highlights

Striatal sensory responses were studied by whole-cell recordings and optogenetics
Dopamine (DA) depletion affects intrinsic and sensory properties in direct pathway neurons
The encoding of bilateral tactile stimuli is impaired following DA depletion
Administration of L-DOPA can correct sensory deficits caused by DA depletion.
for more see: https://doi.org/10.1016/j.neuron.2017.05.004
This study came to my attention the researchers used our Enkaphalin Antibody as a marker for the Dopaminergic Neurons. 
Image: Mouse striatum stained with D2 cell marker Enkephalin (RA14124) in green and with neuronal marker NeuN in red courtesy of Dr Heike Rebholz of City College of New York

Friday, May 19, 2017

TRPV1 Channels and Neuropathic Pain

Neuromics' TRPV1 Stain Neurons and Microglia for Study

TRPV1 is mainly functional in the microglia. Its activation, beyond controlling microglia reaction per se, modulated microglia-neuron communication, by promoting release of extracellular vesicles (EVs) from microglia. Indeed, EVs are important mediators of intercellular communication between microglia and brain cells: Maria Cristina Marrone, Annunziato Morabito, Michela Giustizieri, Valerio Chiurchiù, Alessandro Leuti, Marzia Mattioli, Sara Marinelli, Loredana Riganti, Marta Lombardi, Emanuele Murana, Antonio Totaro, Daniele Piomelli, Davide Ragozzino, Sergio Oddi, Mauro Maccarrone, Claudia Verderio & Silvia Marinelli. TRPV1 channels are critical brain inflammation detectors and neuropathic pain biomarkers in mice. Nature Communications 8, Article number: 15292 (2017) doi:10.1038/ncomms15292.

(a–f) Sections of cortical tissue from WT and TRPV1−/− mice, fixed after exposure to ACSF (a,d), ACSF plus vehicle (DMSO; b,e) and ACSF plus 1μM capsaicin (c,f) and immune-processed for iba-1 to stain microglia cells (in red). INSETs are zoom images taken from an area delimited by the yellow square for each condition. (g), Bar graph of percentage of cortical microglia cell phenotype (resting, ameboid, bushy and hypertrophied), in control (grey bars), vehicle- (dark grey bars) and capsaicin- treated (red bars) cortical sections from WT mice. Capsaicin treatment causes a significant shift from ramified and bushy to hypertrophied morphology. (h), Same as in ‘g’ but in cortical sections from TRPV1−/− mice. In these tissues capsaicin fails to induce morphological changes of microglia cells. Note that microglia cells in −/− tissues are already hypertrophied in control conditions (d–f,h).
Our Pain and Inflammation Research Antibodies Continue to be widely used and frequently published.

Monday, May 15, 2017

TRPV1 Antibodies

Designed for Your Success.
The roots of our TRPV1 Antibodies run deep. They have been key to our ongoing success. We have been providing them to Researchers since the inception of Neuromics (12 years ago).

We measure our success one Researcher at a time. Positive feedback includes references in many publications. There are indeed "Tested; Characterized and Research Ready"

Here's a pub hot off the presses: Noémi Bohonyi, Krisztina Pohóczky, Bálint Szalontai, Anikó Perkecz, Krisztina Kovács, Béla Kajtár, Lajos Orbán, Tamás Varga, Sarolta Szegedi, József Bódis, Zsuzsanna Helyes, Miklós Koppán. Local upregulation of transient receptor potential ankyrin 1 and transient receptor potential vanilloid 1 ion channels in rectosigmoid deep infiltrating endometriosis. Molecular Pain. First published date: May-07-2017. 10.1177/1744806917705564.
Figure: Immunohistochemical staining of TRPV1 receptor in healthy eutopic endometrium and in rectosigmoid DIE nodules. (a) Negative control using tris-buffered saline instead of the primary antibody in normal endometrial tissue. (b) Rectal myenteric ganglia, serving as positive control for TRPA1 expression. (c) Healthy eutopic endometrial tissue. (d) Rectosigmoid DIE nodule. (e) Rectosigmoid DIE nodule, glandular component. (f) Rectosigmoid DIE nodule, stromal component. (d) and (f) Sections shown on panels were taken from the same DIE patient who experienced severe, endometriosis associated pain. Background staining was performed with hematoxylin and eosin to reveal the tissue structure. Black arrow heads denote TRPV1 receptor labelling. Magnification is X400, except panel (d) where it is X100. Scale bars: 50 µm, except panel (d) where it is 200 µm.
We frequently post unique data generated by use of our antibodies.

Thursday, May 04, 2017

Culturing Stem Cells in 3-D

Requires Potent Media + Supplements

Neuromics is responding to the many challenges our clients face in building 3-D, in-vivo like, cell- based assays. We do this by offering the most potent Media plus Supplements like FGFS.

Here's a protocol for single cell 3-D assays using hMSCs and Hydrogels. It features use of our ISOKineTM FGF


Images: Cell-centering in cytocompatible microgels enables long-term single-cell 3D culture by preventing cell escape. a) Qualification of Dex-TA microgel crosslinking as a function of the microemulsion flow rate (Qemulsion) and concentration of the H2O2 feed ([H2O2]feed). Blue, green, and red indicate incomplete crosslinking, complete crosslinking, and H2O2 excess, respectively. b,c) Amplex Red assay to quantify the concentration of residual H2O2 ([H2O2]emulsion) in Dex-TA microgel precursor droplets and crosslinked microgels after their retrieval from the diffusion-based crosslinking platform. d) The microencapsulation procedure had no detrimental effect on short-term cell survival. e) Delayed crosslinking resulted in 4 ± 1% cell escape after 7 d of in vitro culture, as compared to 27 ± 5% cell escape when using coupled emulsification and gelation. f) The number of encapsulated cells per microgel tightly followed the Poisson distribution and remained similar throughout long-term (28 d) of in vitro culture, which confirmed that cell centering prevents cell escape. g–i) MSCs encapsulated in delayed enzymatically crosslinked microgels remained viable and metabolically active throughout 28 d of in vitro culture. j) Positive Oil Red O and k) Alizarin Red staining confirmed that l) more than 60% of the microencapsulated MSCs could differentiate into the adipogenic and osteogenic lineage, respectively. Black scale bars: 50 µm, white scale bars: 5 µm. DOI: 10.1002/smll.20160371.

Protocol for Cell Isolation and Expansion: Human MSCs were isolated from fresh bone marrow samples and cultured as previously described. The use of patient material was approved by the local ethical committee of the Medisch Spectrum Twente and informed written consent was obtained for all samples. In short, nucleated cells in the bone marrow aspirates were counted, seeded in tissue culture flasks at a density of 500 000 cells cm−2, and cultured in MSC proliferation medium, consisting of 10% FBS, 100 U mL−1 penicillin, 100 mg mL−1 streptomycin, 1% GlutaMAX, 0.2 × 10−3 m ascorbic acid, and 1 ng mL−1 bFGF (added fresh) in αMEM. Mouse insulinoma MIN6-B1 cells (provided by Dr. P. Halban, University Medical Center, Geneva, Switzerland) were cultured in MIN6 proliferation medium, consisting of 10% (v/v) FBS, 100 U mL−1 penicillin, and 100 mg mL−1 streptomycin, and 71 × 10−6 m 2-mercaptoethanol (added fresh) in DMEM. When cells reached near confluence, the cells were detached using 0.25% Trypsin-EDTA at 37 °C and subsequently subcultured or used for experimentation.

I am at your beck and call to answer questions on our Cell Based Assay Solution. Pete Shuster-CEO and Owner, direct phone: (612) 801-1007 or pshuster@neuromics.com.

Tuesday, April 25, 2017

Got Autofluorescence?

Problem Solved!

Autofluorescence muddies data and can lead to incorrect solutions. Using our FluoMateTM  ,you can trust your results. Check it out today.

FluoMute™ ready-to-use reagent to reduce autofluorescence in cells and tissue. Just incubate fixed cells of tissue sections with FluoMute™ for 30-60 min at room temperature, rinse with PBS and continue with immunofluorescence ICC or/and IHC protocols. Treatment with FluoMute™ does not affect cell morphology and the integrity of tissue antigens to be detected with primary antibodies. FluoMute™ is compatible with paraffin-embedded and frozen tissue sections, stem cells, lymphocytes and mammalian cell lines of different origin.

Wednesday, April 19, 2017

Hypoxia Induced Angiogenesis and Tumor Microenvironment

Neuromic's HUVECS Used in Study

The tumor microenvironment is essential for promoting tumor physiology, structure, function, and growth. It is important that emerging therapies eradicate both tumors and related microenvironment. This important study focuses on the formation of these microenvironments: ERICA K. SCHNETTLER. THE FUNCTIONAL ROLE OF MIR-210 IN HYPOXIA-INDUCED ANGIOGENESIS. A DISSERTATION SUBMITTED TO THE FACULTY OF THE UNIVERSITY OF MINNESOTA. FEBRUARY 2017...Primary Human umbilical vein endothelial cells (HUVEC) were purchased from Lonza (Basel, Switzerland) and Neuromics (Edina, MN)...



Figure: miR-210 sensitizes HUVECs to bFGF induced tube formation. (A)Representative images of HUVEC tube formation are shown at 10X magnification. Cells were treated with miR-210 or sc-miR, serum starved, and then plated on a Geltrex (reduced growth factor) layer in the presence or absence or bFGF to stimulate tube formation. (B) Histogram represents quantification of total tube length, number of nodes, and junctions in the tube formation assay described in A. Analysis done with ImageJ Angiogenesis Analyzer plugin.

We will continue to post our updates our primary Human Endothelial Cells as they develop.

Thursday, April 13, 2017

mGluRs Protect OPCs

Valuable for Remyelination of Damaged Neurons

We add a new publication to our mGluR Markers Category: Arthur M. Butt, Ilaria Vanzulli, Maria Papanikolaou, Irene Chacon De La Rocha, Virginia E. Hawkins. Metabotropic Glutamate Receptors Protect Oligodendrocytes from Acute Ischemia in the Mouse Optic Nerve. Neurochem Res (2017). doi:10.1007/s11064-017-2220-1. Its focus is the protective characteristics of mGluRs.


Images: Expression of mGluR in optic nerve oligodendrocytes. a RT-qPCR of mGluR subtypes in the postnatal (P8–12) and young adult (P30–35) optic nerve, compared to cortex at the same ages (inset); data are expressed as mean ± SEM ΔΔCT relative to GAPDH, ***p < 0.001 determined by ANOVA and post hoc Bonferroni’s test. b, c Oligodendrocytes in optic nerve explant cultures from P8 PLP-DsRed reporter mice after 10 DIV were immunolabelled for mGluR2/3 (d) and mGluR5 (e), illustrating single channels (Di, Dii, Ei, Eii) and the merged channel in which mGluR colocalization with PLP appears white (Diii, Eiii); scale bars 10 µm

Thursday, April 06, 2017

Need the Beat?

Check out our Cardiomyocytes!
We are pleased to announce the addition of rat and mouse myocytes to our extensive catalog of primary and stem cells.

Questions? Do not hesitate to contact me directly at pshuster@neuromics.com or 612-801-1007. Thank you. Pete Shuster, CEO and Owner

Friday, March 31, 2017

Immuno-fluorescence in 3-D

Potent Markers!

We are seeing more 3-D Cell Based Assays being used for Neuroscience Research. It is important researchers have the Neuron-Astroglial-Progenitor Markers required for staining in 3-D. This helps researchers determine the cell types present in their assays.

I have posted here published results. I would like to share the latest: Yiting Liu, Katherine S. Given, Danielle E. Harlow, Adeline M. Matschulat, Wendy B. Macklin, Jeffrey L. Bennett and Gregory P. Owens. Myelin-specific multiple sclerosis antibodies cause complement-dependent oligodendrocyte loss and demyelination. Acta Neuropathologica Communications Neuroscience of Disease 20175:25
DOI: 10.1186/s40478-017-0428-6



3D movie reconstructed by super-resolution structured illumination microscopy (SIM) imaging of live organotypic mouse cerebellar slices stained with MS#30 (red), then fixed and stained for MAG (blue) and NF-H (purple). MS#30 reactivity was on oligodendrocyte processes, including those contacting adjacent axons, and on myelinated MAG+ axons, outside of MAG layer. Scale bar: 2 μm. (MPG 90340 kb).
We will continue to post cool applications for our antibodies here.

Sunday, March 26, 2017

Targeted Delivery of Our UCB Derived hMSCs

Liver-targeting Delivery via Intravenous Injection of Cells

Check out how our UCB Human Mesenchymal Stem Cells are engineered for delivery to the liver: Hahn, Sei Kwang (Pohang-si, KR), Kim, Yun Seop (Seoul, KR), Kong, Won Ho (Pohang-si, KR),Kim, Hyemin (Daegu, KR). HYALURONIC ACID DERIVATIVES AND COMPOSITION FOR CELL-SURFACE ENGINEERING USING THE SAME. United States Patent Application 20170067012.
Images: Neuromics' hMSCS in culture
Preparation method of a hyaluronic acid derivative capable of modifying the surface of cells and also having biocompatibility, biodegradability, and liver-targeting deliver property, and use of the hyaluronic acid derivative prepared thereby as a liver-targeting cell delivery system.

Saturday, March 18, 2017

High Titer Cathepsin Antibodies

Used in Thyroid Gland Research

We strive to provide quality tools to study proteases and apoptosis. Here is a publication featuring 2 of our Cathepsin Antibodies: Jonas Weber, Joseph McInnes, Cise Kizilirmak, Maren Rehders, Maria Qatato, Eva K. Wirth, Ulrich Schweizer, Francois Verrey, Heike Heuer, Klaudia Brix. Interdependence of thyroglobulin processing and thyroid hormone export in the mouse thyroid gland. European Journal of Cell Biology. Available online 6 March 2017. doi.org/10.1016/j.ejcb.2017.02.002... goat anti-cathepsin B (GT15047; 1 in 1000, Neuromics through Acris, Herford, Germany), goat anti-cathepsin L (GT15049; 1 in 1000, Neuromics through Acris)...

Images: Protein levels of cathepsin B, D, and L in thyroids of TH transporter-deficient adult mice. Whole thyroid lysates of adult mice (5–8 months old) were separated on horizontal SDS-gels, transferred to nitrocellulose and incubated with antibodies against cathepsins B, D or L (left panels). Densitometry of the indicated bands revealed that cathepsin D protein levels were elevated significantly in Mct8/Mct10-deficient mice, whereas cathepsin B and L levels were increased in all investigated genotypes when compared to WT (right panels). 

Images: Expression and localization of cathepsin B in thyroid glands from TH transporter-deficient mice. Cathepsin B (white, red) was mainly localised in vesicles of thyrocytes of WT (A) and Mct10- (B) Mct8- (C), and Mct8/Mct10-deficient (D) animals but also associated with the apical plasma membrane domain and within the lumen of thyroid follicles (E to H, asterisks). Thyroid tissue taken from cathepsin B-deficient animals served as controls for antibody specificity, which was confirmed by lack of primary antibody reactivity (I). Vesicular staining (arrows) of cathepsin B is more pronounced and signal intensities (J) are slightly increased in both, Mct8- (G) or Mct8/Mct10-deficient (H) mouse thyroids when compared to WT (E). Representative images of 3 animals (5–8 months old) per genotype are displayed.

We will continue to post relevant stories of our markers in action.

Monday, March 13, 2017

Certified and Potent FBS

We Use It for our Primary, Human Cell Culture Media

We have a low introductory Fetal Bovine Serum price for this week only (3/13-3/19)=$299/500 ml.


HRMECs were initiated by elutriation from dissociated normal human retinal tissue. Passage 3 cells are ship in proliferating culture with a confluency of greater than 90 %. ENDO-Growth medium containing 5% serum and growth supplements are recommended for culture. Cells have an average additional population doubling levels >16 when cultured.

Monday, March 06, 2017

Adult Primary Neurons

Build Yourself a Stock. We now have adult primary neurons that can be passaged up to 5 times! You can now build a stock of 20-30 million cells.
Human primary neurons are isolated from brain cortical tissue. We highly recommend culturing in our human neuron growth media (cat#HNM001).
Check out our many Primary Neuron and Astrocyte options.

ECS Derived hN2 Human Primary Neurons grown in culture for 4 days and stained with our chicken polyclonal to Neurofilament light or low molecular weight chain NF-L, a marker of neurons. Many of the differentiating cells show strong cytoplasmic and clearly fibrillar staining for NF-L. Blue stain is DAPI and reveals cell nuclei of some nonneuronal cells in these cultures.
Check out related Markers!
MO22110
Mouse IgG
H; M; R
IF; WB
100 ul
$245
MO15055
Mouse IgG
H; M; R
WB
100 ug
$255
MO22113
Mouse IgG
B; H; M; P; R
IF; WB
100 ul
$245
RA22113
Chicken IgY
H; M; R
IF; IHC; WB
100 ul
$245
MO30000
Mouse IgG
H; M; P
IHC
50 ul
$365
RA22105
Rabbit IgG
Ca; Ch; H; M; R
ICC; IHC; WB
100 ul
$275
CH22111
Chicken IgY
Ca; H; M; R
IHC
100 ul
$245
MO22111
Mouse IgG
H; M; R
IF; WB
100 ul
$245
CH22113
Rabbit IgG
H; R
IF; WB
100 ul
$245







Wednesday, March 01, 2017

Staining Tissue From Space Mice

Our Synaptic Marker is Used to Compare Earth vs Space Samples
Exposure to the microgravity conditions of spaceflight alleviates the load normally imposed by the Earth’s gravitational field upon the inner ear utricular epithelia. Previous ultrastructural investigations showed that spaceflight induced an increase in synapse density within hair cells of the rat utricle. However, the utricle exhibits broad physiologic heterogeneity across different epithelial regions, and it is unknown whether capabilities for synaptic plasticity generalize to hair cells across its topography. To achieve systematic and broader sampling of the epithelium than previously conducted we used immunohistochemistry and volumetric image analyses to quantify synapse distributions across representative utricular regions in specimens from mice exposed to spaceflight (a 15-day mission of the space shuttle Discovery). These measures were compared to similarly-sampled Earth-bound controls. Following paraformaldehyde fixation and microdissection, immunohistochemistry was performed on intact specimens to label presynaptic ribbons (anti-CtBP2) and postsynaptic receptor complexes (anti-Shank1A) DOI: 10.1152/jn.00240.2016.

Mature vestibular hair cells retain capabilities for structural plasticity manifested through modulation of synapse density. Investigations are ongoing that are testing the hypothesis that synapse density increases may result from exposure to centrifugation-induced hypergravity, which would provide the foundation for future research into the molecular mechanisms through which these modifications are induced. This research will provide insight and strategies for inner ear rehabilitation through the induction of synapse density increases in conditions of vestibular paresis.

Maybe zero gravity will play a role in therapies for hearing loss?

Monday, February 20, 2017

Holistic Medicine for the Brain

Mind Expansion? 

There is a slowly growing body of support for certain hallucinogenic serotonin-like molecules supporting cognitive gains, antidepressant effects and changes in brain areas related to attention, self-referential thought, and internal mentation. These molecules are present in Virola Ayahuasca and used in traditional native South American medicine.

Here researchers found that in silico systems biology analyses support 5- MeO-DMT’s anti-inflammatory effects and reveal a modulation of proteins associated with the formation of dendritic spines, including proteins involved in cellular protrusion formation, microtubule dynamics and cytoskeletal reorganization. Proteins involved in long-term potentiation were modulated in a complex manner, with significant increases in the levels of NMDAR, CaMKII and CREB, but a reduction of PKA and PKC levels. These results offer possible mechanistic insights into the neuropsychological changes caused by the ingestion of substances rich in dimethyltryptamines: Vanja Dakic, Juliana Minardi Nascimento, Rafaela Costa Sartore, Renata de Moraes Maciel, Draulio B. de Araujo, Sidarta Ribeiro, Daniel Martins-de-Souza , Stevens Rehen. Short term changes in the proteome of human cerebral organoids induced by 5-methoxy-N,N-dimethyltryptamine. bioRxiv preprint first posted online Feb. 13, 2017; doi: http://dx.doi.org/10.1101/108159... anti-5-HT2A (RA24288, Neuromics)...
Images: Cerebral organoids express 5-MeO-DMT receptors and different cell type markers (A) Cerebral organoids presenting smooth texture and homogeneous coloring at 45 days of differentiation (scale bar 1000 µm). (B) Cerebral organoids are not peer-reviewed) is the author/funder. It is made available under a CC-BY-NC-ND 4.0 International license. bioRxiv preprint first posted online Feb. 13, 2017; doi: http://dx.doi.org/10.1101/108159. The copyright holder for this preprint (which was 8 composed by several cell types, including mature neurons, as shown by MAP2 staining. (C) Cells expressing AMPAR1 are found in the organoid edge, while (D) cells expressing NMDAR1 and (E) GFAP are detected within the organoid. (F) Cells positive for 5-HT2A receptor, and (G) σ-1R, the primary molecular targets for 5-MeODMT, are also found in the organoid. Scale bars: A = 1000 µm; B = 50 µm; C, D, E, F, and G = 20 µm. (H) The expression of molecular targets for 5-MeO-DMT was also confirmed by RT-PCR.



Dimethyltryptamines should be studied further as potential therapies for depression and related disorders.

Monday, February 13, 2017

Human Melanoma Cancer Associated Fibroblasts

More Hard to Find Human Cells
We are recognized for providing potent, pure and easy to culture CAFs and Immortalized Tumor Cells. We are pleased to announce the addition of Melanoma CAFS. Our introductory price is only 899 USD/1,000,000 Cells. They have been successfully passaged 10X.
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Image: Human Melanoma Cells in Culture
Need CAFs or Tumor Cells? Just email me at pshuster@neuromics.com.

Tuesday, January 31, 2017

Desperately Seeking Data

Answering the Bell
We continue to seek data using our cells. We offer a reward of 25 USD Starbucks' Gift Card.

We were pleased to receive a recently published study from Dr. Mahendran Subramanian of Keele University. In this study, researchers showed that oscillating nanomagnetic gene transfection could be used to successfully transfect SH‐SY5Y cells as well as our primary hippocampal and cortical neurons on different days in vitro. This novel technique was used to effectively deliver genetic material into various cell types, resulting in high transfection efficiency and viability. Mahendran Subramanian, Aimee‐Jayne Tyler, Eva Maria Luther, Elena Di Daniel, Jenson Lim and Jon Dobson. Oscillating Magnet Array−Based Nanomagnetic Gene Transfection: A Valuable Tool for Molecular Neurobiology Studies. Nanomaterials 2017, 7, 28; doi:10.3390/nano7020028...Primary rat hippocampal and cortical neurons were obtained from Neuromics (Edina, MN, USA) and disassociated using papain disassociation kit (Worthington, NJ, USA) according to the manufacturer’s instructions. Isolated neurons were maintained using neurobasal medium supplemented with 5% FBS, 0.5 mM Glutamax, 2% B27 supplement, 25 μM L‐glutamine and seeded onto poly‐D‐lysine–coated cells culture plates...
Figure 1. Oscillating magnet array−based nanomagnetic gene transfection experimental setup. (A) Representation of a 96‐well oscillating magnet array–based nanomagnetic transfection setup using NdFeB magnetic array (nanotherics); (B) Dimensions of the permanent magnets and magnetostatic (vectorpotential) algorithm based magnetic field density |B| distribution (T) contour plot for the NdFeB magnetic array.

Figure 2. Gene delivery by oscillating nanomagnetic gene transfection in primary cortical neurons. Images of pmaxGFP plasmid expressed in primary neurons using fluorescence microscopy and its corresponding Hoechst 33,342 stained counterpart of transfected DIV 1 (A,C) and DIV 5 (B,D) mature neurons were taken 48 h post transfection.

If you have data to share email it to me, pshuster@neuromics.com and we'll email you a 25 USD gift card. Thank you. Pete Shuster, CEO & Owner.

Saturday, January 28, 2017

mCherry and GFP

Excellent Markers

These markers are stout fluorescent tracers for transfection and transgenic experiments. Here is data showing our mCherry Mouse Monoclonal Antibody Staining transfected HeLa Cells.

Image: Blot of HEK293 cells transfected with pFin-EF1-mCherry vector, courtesy of the Semple-Rowland lab at the University of Florida. There is a strong clean band at about 30 kDa. HEK293 cells which were not transfected with this vector show no protein bands.

As with all our products, if you are not 100% satisfied, we refund your purchase with no questions asked.

Saturday, January 21, 2017

Leptin and Remyelination

Leptin Promotes Proliferation of OPCs

Demyelination occurs in many diseases of the Central Nervous System (CNS) including Multiple Sclerosis and Parkinson's Disease. Here researchers show that Leptin plays a role in the proliferation of Oligodendrocyte Precursor Cells (OPCs): These cells are critical for keeping the myelin sheath on Neurons of the CNS healthy and happy.  Ken Matoba, Rieko Muramatsu & Toshihide Yamashita. Leptin sustains spontaneous remyelination in the adult central nervous system. Scientific Reports 7, Article number: 40397 (2017) doi:10.1038/srep40397.

Our LepRB Antibody is used in this study to stain OPCs.


Figures: (a) Representative image of cultured OPCs stained with antibodies against LepRb (green) and PDGFRα (red). Scale bar: 25 μm. (b) Relative BrdU incorporation into the OPC obtained from the brain (left graph) and spinal cord (right graph). Cells were treated with recombinant leptin for 48 h (n = 4). (Left graph) P = 0.005993 (control vs 10 ng/mL), 0.045616 (control vs 100 ng/mL), (Right graph) P = 0.004456 (control vs 10 ng/mL), 0.017859 (control vs 100 ng/mL). (c) Relative BrdU incorporation into the OPC after leptin stimulation (10 ng/ml) with U0126 (20 μM), a MEK inhibitor (n = 4 for brain OPCs, n = 3 for spinal cord OPCs). (Left graph) P = 0.019753 (control vs leptin), 0.039433 (leptin vs leptin + U0126), (Right graph) P = 0.045545 (control vs leptin), 0.04486 (leptin vs leptin + U0126). (d) Representative images of western blotting (upper panels) and quantitative analysis of ERK phosphorylation (lower graph) are shown. OPCs were treated with leptin (10 ng/ml) under indicated periods (n = 3). P = 0.006352 (2 min), 0.016571 (5 min), 0.017675 (10 min), 0.024100 (15 min), 0.081342 (30 min).
We are in the process of looking for Labs to sponsor Neuromics' to isolate and purify adult human OPCs in return for receiving 2,000,000 cells. Stay tuned.

Friday, January 13, 2017

Rising FBS Prices Raising Your Costs?

Give us a shot

Fetal Bovine Serum (FBS) is the most highly used growth factor in cell culture due to its high level of nutrients. Our FBS is produced to the highest standards in order to reduce risk and product variability and to ensure product safety and performance. Our FBS is 9CFR-tested, meeting FDA and USDA requirements. Fetal bovine serum products can also be tested to meet EMEA requirements.

Note: We test each lot of FBS on our primary human cell cultures enabling us to choose lots yielding the best results...Testimonial: "We have used the FBS from Neuromics in feeding media for primary mouse astrocytes as well as for some cell lines. Your product is good and we plan to continue using it.” - Svetlana Vidensky, MS, Senior Research Specialist in Dr. Jeffrey Rothstein lab, Department of Neurology, Johns Hopkins University


100 ml trial size is available for only $149. Contact me at 612-801-1007 or pshuster@neuromics.com to order the trial size. We also offer 100% money back guarantee should we not meet your expectations. Pete Shuster-CEO and Owner Neuromics