6 research outputs found
Additional file 1 of Lateralized response of skull bone marrow via osteopontin signaling in mice after ischemia reperfusion
Additional file 1. Table S1. Detailed animal characteristics; Table S2. List of antibodies for flow cytometry and Immunofluorescence; Fig. S1. a Gating strategy for the flow cytometry assay. b Neutrophil-to-monocyte ratio between the ipsilateral and contralateral groups in the bone marrow of male mice. The data are presented as the means ± SD (paired t test, *P < 0.05, n=6-7). c Comparison of neutrophils between ipsilateral and contralateral groups in the bone marrow of different tissues of female mice. The data are presented as the means ± SD (paired t test, **P < 0.01, n=6). d Comparison of monocytes between ipsilateral and contralateral groups in the bone marrow of different tissues of female mice. The data are presented as the means ± SD (paired t test, **P < 0.01, n=6). e Neutrophil-to-monocyte ratio between ipsilateral and contralateral skull marrow of female mice. The data are presented as the means ± SD. (paired t test, **P < 0.01, n=6); Blot images and X-ray image of array
Nanoplatform Assembled from a CD44-Targeted Prodrug and Smart Liposomes for Dual Targeting of Tumor Microenvironment and Cancer Cells
The tumor microenvironment (TME)
plays a critical role in tumor initiation, progression, invasion,
and metastasis. Therefore, a therapy that combines chemotherapeutic
drugs with a TME modulator could be a promising route for cancer treatment.
This paper reports a nanoplatform self-assembled from a hyaluronic
acid (HA)-paclitaxel (PTX) (HA-PTX) prodrug and marimastat (MATT)-loaded
thermosensitive liposomes (LTSLs) (MATT-LTSLs) for the dual targeting
of the TME and cancer cells. Interestingly, the prodrug HA-PTX can
self-assemble on both positively and negatively charged liposomes,
forming hybrid nanoparticles (HNPs, 100 nm). Triggered by mild hyperthermia,
HA-PTX/MATT-LTSLs HNPs rapidly release their payloads into the extracellular
environment, and the released HA-PTX quickly enters 4T1 cells through
a CD44-HA affinity. The HNPs possess promoted tumor accumulation (1.6-fold),
exhibit deep tumor penetration, and significantly inhibit the tumor
growth (10-fold), metastasis (100%), and angiogenesis (10-fold). Importantly,
by targeting the TME and maintaining its integrity <i>via</i> inhibiting the expression and activity of matrix metalloproteinases
(>5-fold), blocking the fibroblast activation by downregulating
the TGF-β1 expression (5-fold) and suppressing the degradation
of extracellular matrix, the HNPs allow for significant metastasis
inhibition. Overall, these findings indicate that a prodrug of an
HA–hydrophobic-active compound and liposomes can be self-assembled
into a smart nanoplatform for the dual targeting of the TME and tumor
cells and efficient combined treatment; additionally, the co-delivery
of MATT and HA-PTX with the HNPs is a promising approach for the treatment
of metastatic cancer. This study creates opportunities for fabricating
multifunctional nanodevices and offers an efficient strategy for disease
therapy
Nanoplatform Assembled from a CD44-Targeted Prodrug and Smart Liposomes for Dual Targeting of Tumor Microenvironment and Cancer Cells
The tumor microenvironment (TME)
plays a critical role in tumor initiation, progression, invasion,
and metastasis. Therefore, a therapy that combines chemotherapeutic
drugs with a TME modulator could be a promising route for cancer treatment.
This paper reports a nanoplatform self-assembled from a hyaluronic
acid (HA)-paclitaxel (PTX) (HA-PTX) prodrug and marimastat (MATT)-loaded
thermosensitive liposomes (LTSLs) (MATT-LTSLs) for the dual targeting
of the TME and cancer cells. Interestingly, the prodrug HA-PTX can
self-assemble on both positively and negatively charged liposomes,
forming hybrid nanoparticles (HNPs, 100 nm). Triggered by mild hyperthermia,
HA-PTX/MATT-LTSLs HNPs rapidly release their payloads into the extracellular
environment, and the released HA-PTX quickly enters 4T1 cells through
a CD44-HA affinity. The HNPs possess promoted tumor accumulation (1.6-fold),
exhibit deep tumor penetration, and significantly inhibit the tumor
growth (10-fold), metastasis (100%), and angiogenesis (10-fold). Importantly,
by targeting the TME and maintaining its integrity <i>via</i> inhibiting the expression and activity of matrix metalloproteinases
(>5-fold), blocking the fibroblast activation by downregulating
the TGF-β1 expression (5-fold) and suppressing the degradation
of extracellular matrix, the HNPs allow for significant metastasis
inhibition. Overall, these findings indicate that a prodrug of an
HA–hydrophobic-active compound and liposomes can be self-assembled
into a smart nanoplatform for the dual targeting of the TME and tumor
cells and efficient combined treatment; additionally, the co-delivery
of MATT and HA-PTX with the HNPs is a promising approach for the treatment
of metastatic cancer. This study creates opportunities for fabricating
multifunctional nanodevices and offers an efficient strategy for disease
therapy
Image_2_Role of complement C1q/C3-CR3 signaling in brain injury after experimental intracerebral hemorrhage and the effect of minocycline treatment.tif
AimThe complement cascade is activated and may play an important pathophysiologic role in brain injury after experimental intracerebral hemorrhage (ICH). However, the exact mechanism of specific complement components has not been well studied. This study determined the role of complement C1q/C3-CR3 signaling in brain injury after ICH in mice. The effect of minocycline on C1q/C3-CR3 signaling-induced brain damage was also examined.MethodsThere were three parts to the study. First, the natural time course of C1q and CR3 expression was determined within 7 days after ICH. Second, mice had an ICH with CR3 agonists, LA-1 or vehicle. Behavioral score, neuronal cell death, hematoma volume, and oxidative stress response were assessed at 7 days after ICH. Third, the effect of minocycline on C1q/C3-CR3 signaling and brain damage was examined.ResultsThere were increased numbers of C1q-positive and CR3-positive cells after ICH. Almost all perihematomal C1q-positive and CR3-positive cells were microglia/macrophages. CR3 agonist LA-1 aggravated neurological dysfunction, neuronal cell death, and oxidative stress response on day 7 after ICH, as well as enhancing the expression of the CD163/HO-1 pathway and accelerating hematoma resolution. Minocycline treatment exerted neuroprotective effects on brain injury following ICH, partly due to the inhibition of C1q/C3-CR3 signaling, and that could be reversed by LA-1.ConclusionsThe complement C1q/C3-CR3 signaling is upregulated after ICH. The activation of C1q/C3-CR3 signaling by LA-1 aggravates brain injury following ICH. The neuroprotection of minocycline, at least partly, is involved with the repression of the C1q/C3-CR3 signaling pathway.</p
Image_1_Role of complement C1q/C3-CR3 signaling in brain injury after experimental intracerebral hemorrhage and the effect of minocycline treatment.tif
AimThe complement cascade is activated and may play an important pathophysiologic role in brain injury after experimental intracerebral hemorrhage (ICH). However, the exact mechanism of specific complement components has not been well studied. This study determined the role of complement C1q/C3-CR3 signaling in brain injury after ICH in mice. The effect of minocycline on C1q/C3-CR3 signaling-induced brain damage was also examined.MethodsThere were three parts to the study. First, the natural time course of C1q and CR3 expression was determined within 7 days after ICH. Second, mice had an ICH with CR3 agonists, LA-1 or vehicle. Behavioral score, neuronal cell death, hematoma volume, and oxidative stress response were assessed at 7 days after ICH. Third, the effect of minocycline on C1q/C3-CR3 signaling and brain damage was examined.ResultsThere were increased numbers of C1q-positive and CR3-positive cells after ICH. Almost all perihematomal C1q-positive and CR3-positive cells were microglia/macrophages. CR3 agonist LA-1 aggravated neurological dysfunction, neuronal cell death, and oxidative stress response on day 7 after ICH, as well as enhancing the expression of the CD163/HO-1 pathway and accelerating hematoma resolution. Minocycline treatment exerted neuroprotective effects on brain injury following ICH, partly due to the inhibition of C1q/C3-CR3 signaling, and that could be reversed by LA-1.ConclusionsThe complement C1q/C3-CR3 signaling is upregulated after ICH. The activation of C1q/C3-CR3 signaling by LA-1 aggravates brain injury following ICH. The neuroprotection of minocycline, at least partly, is involved with the repression of the C1q/C3-CR3 signaling pathway.</p
Image_3_Role of complement C1q/C3-CR3 signaling in brain injury after experimental intracerebral hemorrhage and the effect of minocycline treatment.tif
AimThe complement cascade is activated and may play an important pathophysiologic role in brain injury after experimental intracerebral hemorrhage (ICH). However, the exact mechanism of specific complement components has not been well studied. This study determined the role of complement C1q/C3-CR3 signaling in brain injury after ICH in mice. The effect of minocycline on C1q/C3-CR3 signaling-induced brain damage was also examined.MethodsThere were three parts to the study. First, the natural time course of C1q and CR3 expression was determined within 7 days after ICH. Second, mice had an ICH with CR3 agonists, LA-1 or vehicle. Behavioral score, neuronal cell death, hematoma volume, and oxidative stress response were assessed at 7 days after ICH. Third, the effect of minocycline on C1q/C3-CR3 signaling and brain damage was examined.ResultsThere were increased numbers of C1q-positive and CR3-positive cells after ICH. Almost all perihematomal C1q-positive and CR3-positive cells were microglia/macrophages. CR3 agonist LA-1 aggravated neurological dysfunction, neuronal cell death, and oxidative stress response on day 7 after ICH, as well as enhancing the expression of the CD163/HO-1 pathway and accelerating hematoma resolution. Minocycline treatment exerted neuroprotective effects on brain injury following ICH, partly due to the inhibition of C1q/C3-CR3 signaling, and that could be reversed by LA-1.ConclusionsThe complement C1q/C3-CR3 signaling is upregulated after ICH. The activation of C1q/C3-CR3 signaling by LA-1 aggravates brain injury following ICH. The neuroprotection of minocycline, at least partly, is involved with the repression of the C1q/C3-CR3 signaling pathway.</p