Sickle RBCs Stimulate Human Monocyte Cytokine Expression.

Abstract Sickle red cells (SS RBCs) express numerous adhesion molecules, including LW, CD44, CD47, and Lutheran (LU) proteins, as well as phosphatidylserine. Proadhesive SS RBCs bind to endothelial cells, leading to their activation. Sickle monocytes have also been shown to express increased surface CD11b, as well as the cytokines tumor necrosis factor α (TNF-α) and interleukin 1β (IL-1β), indicating their activated state. Chronic inflammation and high plasma levels of IL-1β can stimulate leukocyte proliferation and leukocytosis. An association between leukocytosis and increased morbidity and mortality of sickle cell disease (SCD) has been observed. However, the mechanism of monocyte activation in SCD is still unknown. We therefore sought to determine if SS RBCs played a role in monocyte activation. Blood samples were obtained from six normal adult volunteers, and SS RBCs were obtained from 12 adult patients homozygous for hemoglobin S. Plasma and buffy coat were removed, and 6 μl of SS RBCs were washed with sterile phosphate-buffered saline. After incubation with one million cells of the human promonocytic cell line U937 for 2 hours at 37°C, RBCs were lysed and total U937 RNA was isolated. Following reverse transcription, real-time PCR was performed using 200 nM primers for IL-1β, IL-6 or TNF-α, 50 ng cDNA and 12.5 μl of SYBR green 2× Super Mix in a 25 μl reaction volume. The amplification reaction was carried out over 40 cycles (10 min at 95°C, followed by a two-step cycling program of 15s at 95°C and 30s at 60°C). GAPDH was analyzed in parallel as an internal control. IL-1β, IL-6 and TNF-α U937 mRNA was significantly up-regulated after incubation with SS RBCs vs incubation with normal RBCs (relative to control without RBCs, relative mRNA levels: IL-1β: 2.77 ± 1.79 vs 0.82 ± 0.19, p=0.012; IL-6: 2.17 ± 0.94 vs 0.74 ± 0.34, p=0.003; and TNF-α: 3.01 ± 1.30 vs 1.09 ± 0.17, p=0.003). To identify the adhesion molecules involved in the interaction between SS RBCs and monocytes, 10 μg/ml soluble recombinant Lutheran (srLU) was incubated with U937 cells at 37°C for 2h. After incubation, total RNA was isolated from untreated and treated U937 cells. Real time PCR results showed that srLU treatment activated U937 cell TNF-α expression, (relative mRNA level 1.63 ± 0.02 vs 1.00 ± 0.01, p<0.0001, n=3) but not IL-1β or IL-6 expression (relative mRNA levels sLU treated vs untreated control, n=3-IL-1β: 1.24 ± 0.09 vs 1.00 ± 0.02, p=0.07; IL-6: 1.35 ± 0.30 vs 1.00 ± 0.01, p = 0.31). Neither soluble LW nor soluble CD44 had a similar effect. To verify that LU was involved in the interaction between SS RBCs and monocytes, inhibition assays were also performed. SS RBCs were incubated with anti-LU Ab for 1 h at 4°C to block RBC surface LU before incubation with U937 cells. Data from five paired treated and untreated samples showed decreased TNF-α mRNA expression after anti-LU antibody treatment (1.16 ± 0.14 vs 1.40 ± 0.12, p=0.005). Overall, these data suggest that monocytes can be activated by cell-cell interactions with SS RBCs to express the cytokines IL-1β, IL-6 and TNF-α. This activation is at least partially mediated through SS RBC Lutheran protein, which is over-expressed by these cells and is known to bind to leukocyte α4β1 integrin. These studies thus reveal that intact SS RBCs likely play a direct role in monocyte activation in SCD patients.

Download Full-text

Genome-wide screening of m6A-modified transcript in the Wilms’ tumor

10.21203/rs.3.rs-197376/v1 ◽

2021 ◽

Author(s):

Zhuo Liu ◽

Feng He ◽

Jing Liu ◽

Shengrong OuYang ◽

Zexi Li ◽

...

Keyword(s):

Gene Ontology ◽

Real Time ◽

Real Time Pcr ◽

Wilms Tumor ◽

Expression Patterns ◽

Mrna Levels ◽

Gene Ontology Analysis ◽

Quantitative Real Time Pcr ◽

Related Factors ◽

Significant Difference

Abstract Background Wilms’ tumor, also called nephroblastoma, is the most common pediatric renal malignancy. The pathogenesis of Wilms’ tumor has been attributed to several genetic and epigenetic factors. However, the most pervasive internal mRNA modification that affects almost every process of RNA metabolism, RNA N6-Methyladenosine (m6A) methylation, has not been characterized in Wilms’ tumor. Methods Wilms’ tumor (WT) and adjacent non-cancerous (NC) tissue samples were obtained from 23 children with nephroblastoma, and the global m6A levels were measured by mass spectrometry. Analyses by m6A-mRNA epitranscriptomic microarray and mRNA microarray were performed, and m6A-related mRNAs were validated by quantitative real-time PCR for input and m6A-immunoprecipitated RNA samples from WT and NC tissues. Gene ontology analysis and KEGG pathway analysis were performed for differentially expressed genes, and expression of RNA methylation-related factors was measured by quantitative real-time PCR. Results The total m6A methylation levels in total RNA of WT samples and NC samples were (0.21 ± 0.01)% and (0.22 ± 0.01)%, respectively, with no statistically significant difference. Fifty-nine transcripts were differentially m6A-methylated between the WT and NC groups, which showed distinct m6A modification patterns. Gene ontology analysis indicated that m6A-modified genes were enriched in cancer-associated pathways, including the mTOR pathway, and conjoint analysis of the unique methylation and gene expression patterns in WT samples suggested an association with metabolic pathways.The mRNA levels of the m6A-related “reader” genes, YTHDF1, YTHDF2 and IGF2BP3, were statistically higher in WT samples than in NC samples. Conclusion This is the first study to determine the m6A modification profiles in Wilms’ tumor. Our data provide novel information regarding patterns of m6A modification that correlate with carcinogenesis in Wilms’ tumor.

Download Full-text

Cloning, Characterization, and Expression Features of Chicken CDS2 Splicing Variants

10.21203/rs.3.rs-80587/v1 ◽

2020 ◽

Author(s):

Yuanyuan Xu ◽

Shuping Zhang ◽

Yujun Guo ◽

Wen Chen ◽

Yanqun Huang

Keyword(s):

Adipose Tissue ◽

Real Time ◽

Real Time Pcr ◽

Expression Patterns ◽

Mrna Levels ◽

Exogenous Insulin ◽

Quantitative Real Time Pcr ◽

Temporal Expression ◽

Spatio Temporal ◽

The Brain

Abstract Background: The CDS gene encodes the CDP-diacylglycerol synthase enzyme that catalyzes the formation of CDP-diacylglycerol (CDP-DAG) from phosphatidic acid. At present, there are no reports of CDS2 in birds. Here, we identified chicken CDS2 transcripts by combining conventional RT- PCR amplification, 5' RACE (Fig. 1A), and 3' RACE, explored the spatio-temporal expression profiles of total CDS2 and the longest transcript variant CDS2-4, and investigated the effect of exogenous insulin on total the mRNA level of CDS2 by quantitative real-time PCR. Results: Four transcripts of chicken CDS2 (CDS2-1, -2, -3, and -4) were identified, which were alternatively spliced at the 3′-untranslated region (UTR). CDS2 was widely expressed in all tissues examined and the longest variant CDS2-4 was the major transcript. Both total CDS2 and CDS2-4 were prominently expressed in adipose tissue and the heart, and exhibited low expression in the liver and pectoralis of 49 day-old chickens. Quantitative real-time PCR revealed that total CDS2 and CDS2-4 had different spatio-temporal expression patterns in chicken. Total CDS2 exhibited a similar temporal expression tendency with a high level in the later period of incubation (embryonic day 19 [E19] or 1-day-old) in the brain, liver, and pectoralis. While CDS2-4 presented a distinct temporal expression pattern in these tissues, CDS2-4 levels peaked at 21 days in the brain and pectoralis, while liver CDS2-4 mRNA levels were highest at the early stage of hatching (E10). Total CDS2 (P < 0.001) and CDS2-4 (P = 0.0090) mRNA levels in the liver were differentially regulated throughout development of the chicken. Exogenous insulin significantly downregulated the level of total CDS2 at 240 min in the pectoralis of Silky chickens (P < 0.01). Total CDS2 levels in the liver of Silky chickens were higher than that of the broiler in the basal state and after insulin stimulation. Conclusion: Chicken CDS2 has multiple transcripts with variation at the 3′-UTR, which was prominently expressed in adipose tissue. Total CDS2 and CDS2-4 presented distinct spatio-temporal expression patterns, and they were differentially regulated with age in liver. Insulin could regulate chicken CDS2 levels in a breed- and tissue-specific manner.

Download Full-text

Μελέτη της επίδρασης του ενεργοποιού του πλασμινογόνου του τύπου της ουροκινάσης στην παθογένεια της κολίτιδας

10.12681/eadd/37825 ◽

2013 ◽

Author(s):

Ελισάβετ Καραμανάβη

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Ki 67 ◽

Tnf Α ◽

Tgf Β1

Η ύπαρξη συσχέτισης μεταξύ φλεγμονής και καρκίνου είναι πλέον ευρέως αποδεκτή. Τα αποτελέσματα πρόσφατων ερευνών δείχνουν ότι η ανάπτυξη και η επιβίωση των καρκινικών κυττάρων εξαρτώνται σε μεγάλο βαθμό από τους παράγοντες της φλεγμονής. Ορισμένοι ερευνητές θεωρούν τον καρκίνο σαν μια «πληγή» που ο οργανισμός αποτυγχάνει να επουλώσει. Ο ενεργοποιός του πλασμινογόνου του τύπου της ουροκινάσης (uPA) είναι μία πρωτεάση που συμμετέχει τόσο στη φλεγμονή όσο και στην επούλωση. Πολλές εργασίες καταδεικνύουν το ρόλο του συστήματος της ινωδόλυσης στην εξέλιξη, διείσδυση και μετάσταση του καρκίνου, ενώ ο uPA θεωρείται παράγοντας που προάγει την εξέλιξη του καρκίνου. Ωστόσο, δεν υπάρχουν μελέτες που να εξετάζουν τον πιθανό ρόλο του uPA στα πρώιμα στάδια της καρκινογένεσης. Εξαίρεση σε αυτό αποτελεί μία έρευνα, σύμφωνα με την οποία τα Apcmin/+ ποντίκια από τα οποία λείπει το γονίδιο που κωδικοποιεί τον uPA εμφανίζουν λιγότερα αδενώματα στο έντερο. Ο uPA ενεργοποιεί τον Tgf-β1, ο οποίος στα πρώιμα στάδια της καρκινογένεσης έχει ογκο-κατασταλτική δράση. Στόχος της συγκεκριμένης διατριβής ήταν η διερεύνηση της επίδρασης της απουσίας του uPA στην κολίτιδα που προκαλείται από το DSS. Φυσιολογικοί (WT) και uPA-/- BALB/cJ ποντικοί έλαβαν DSS με το πόσιμο νερό. Η νεκροτομή των πειραματόζωων πραγματοποιήθηκε μία εβδομάδα ή επτά μήνες μετά την παύση χορήγησης του DSS. Η φλεγμονή, η ακεραιότητα του επιθηλίου και οι δυσπλαστικές/προ-νεοπλασματικές αλλοιώσεις βαθμονομήθηκαν ξεχωριστά. Σε τομές παραφίνης σημάνθηκαν με ανοσοϊστοχημικά η β-κατενίνη, η Ε-καντχερίνη, ο Tgf-β1, η IL-6 και η IL-17. Για τη σήμανση των κυττάρων σε πολλαπλασιασμό και απόπτωση χρησιμοποιήθηκαν αντισώματα κατά του ki-67 και της κασπάσης-3, αντίστοιχα. Με ανοσοϊστοχημεία σημάνθηκαν επίσης τα Τ-λεμφοκύτταρα, τα ρυθμιστικά Τ-λεμφοκύτταρα, τα μακροφάγα, τα σιτευτικά κύτταρα και τα ουδετερόφιλα. Η ενεργός μορφή του Tgf-β1 και ο uPA προσδιορίστηκαν ποσοτικά στο βλεννογόνο του εντέρου με τη μέθοδο ELISA. Επίσης, χρησιμοποιώντας real-time PCR έγινε ποσοτικός προσδιορισμός των γονιδίων IL-6, IL-10, Tgf-β1, Tgf-βRII και SMAD-4. Τα φλεγμονικά κύτταρα και οι κυτταροκίνες αξιολογήθηκαν ποσοτικά με κατάλληλη μορφομετρική μέθοδο. Επτά μήνες μετά τη χορήγηση του DSS οι πέντε από τους έντεκα (5/11) uPA-/-+DSS ποντικοί εμφάνισαν πολυποειδή αδενώματα, ενώ κανένας από τους WT+DSS ποντικούς δεν εμφάνισε πολύποδα. Επιπλέον, οι uPA-/-+DSS ποντικοί είχαν περισσότερα φλεγμονικά κύτταρα και περισσότερες αλλοιώσεις δυσπλασίας από τους WT+DSS ποντικούς. Προκειμένου να διερευνηθεί γιατί οι uPA-/-+DSS ποντικοί εμφάνισαν πολύποδες, ενώ οι WT+DSS ποντικοί όχι, πραγματοποιήθηκε εξέταση του παχέος εντέρου σε πιο πρώιμη χρονική στιγμή. Μία εβδομάδα μετά τη διακοπή χορήγησης του DSS, και οι δύο ομάδες που έλαβαν DSS εμφάνισαν τις τυπικές αλλοιώσεις της κολίτιδας που προκαλεί το DSS. Ωστόσο, οι uPA-/-+DSS ποντικοί εμφάνισαν περισσότερες διαβρώσεις και πιο προχωρημένου βαθμού αλλοιώσεις δυσπλασίας. Στο βλεννογόνο του παχέος εντέρου των uPA-/-+DSS ποντικών παρατηρήθηκαν περισσότερα ουδετερόφιλα και μακροφάγα, λιγότερα ρυθμιστικά Τ-λεμφοκύτταρα, αύξηση των κυτταροκινών IL-6, IL-17, TNF-α και IL-10 και σημαντική μείωση των επιπέδων του ενεργού Tgf-β1 συγκριτικά με τους WT+DSS ποντικούς. Τα μη λειτουργικά ρυθμιστικά Τ-λεμφοκύτταρα, η πιο επίμονη φλεγμονική αντίδραση και η κληρονομούμενη ανικανότητα παραγωγής επαρκούς ποσότητας ενεργού Tgf-β1 εξωκυτταρικά, λόγω της έλλειψης του uPA, αποτελούν τις πιθανές εξηγήσεις για τη νεοπλασματογένεση που σχετίζεται με τη φλεγμονή στο παχύ έντερο των uPA-/-+DSS ποντικών.

Download Full-text

TLR, RAGE, and HMGB1 in the Inflammatory Response in Ph(-) Myeloproliferative Neoplasm

Blood ◽

10.1182/blood-2020-134988 ◽

2020 ◽

Vol 136 (Supplement 1) ◽

pp. 31-32

Author(s):

Guanfang Shi ◽

Kiron Nair ◽

Preethi Ramachandran ◽

Chi Chen ◽

Ching Wong ◽

...

Keyword(s):

Inflammatory Response ◽

Real Time ◽

Inflammatory Cytokines ◽

Internal Control ◽

Real Time Pcr ◽

Mononuclear Cells ◽

Conflicts Of Interest ◽

Philadelphia Chromosome ◽

Myeloproliferative Neoplasm ◽

Significant Difference

Recent evidence of increased constitutional symptoms and inflammatory cytokines in Philadelphia chromosome negative (Ph (-)) MPN suggests that an inflammatory response is important in the pathogenesis of Ph (-) MPN. Toll-like receptors (TLR), Receptor for Advanced Glycation End products (RAGE) and High mobility group protein B1 (HMGB1) are the important pathways for the inflammatory response. All these three important pathway proteins were studied in MPN diseases in the current studies. Materials and Methods: TLR assay. TLR 2,3, 4, 7, 9 quantification was performed by immuno-staining of 1×106 mononuclear cells (peripheral blood) which were incubated with fluorescence-conjugated anti-TLR-2,3, 4, 7, 9 antibodies and assayed by flow cytometry. HMGB1assay:HMGB1 ELISA kit from Immuno-Biological Laboratories, Inc. (IBL-America) were used. The plasma samples were diluted four times with the provided sample dilution buffer, and assayed in duplicate according to the manufacturer's suggestion. RAGE (RT-PCR) Assay: Total RNA was extracted from normal control or patient mononuclear cells. Predesigned primers for RAGE, and internal control genes were ordered from Qiagen (Germantown, MD). Real-time PCR was performed using SsoAdvanced™ Universal SYBR® Green Supermix (Bio-Rad, Hercules, CA) on Bio-Rad iQ5 Multicolor Real-Time PCR Detection System. At least three house-keeping genes (ribosomal protein L4, TATA box binding protein, and tubulin-α 1b) were used as normalization controls. The expression of RAGE were compared with each internal control. Average of three was used to calculate the ratio of final patient to normal Results: Total of 97 patients with MPN were studied 1) TLR: TLR 3,7,9 was not significantly different from controls. But TLR 2 was significantly increased in both PV, as well as in the MPN group when PV, ET and MF were grouped together as MPN (Fig A). TLR 4 was not significantly increased in PV, ET, MF individually but was found to be significantly increased than the controls, when they are grouped together as MPN (Fig B). 2) RAGE: No significant difference was found between ET, PV, MF individually or when they were grouped together as MPN than the controls (Fig C). 3) HMGB1: No significant difference was seen between ET, PV, MF or when they were grouped as MPN (Fig D). Conclusion: Current study suggests that TLR pathway especially TLR2, and to a lesser extent TLR4 are the important pathways for inflammatory response with increased inflammatory cytokines in MPN, while HMGB1 and RAGE pathways were not different from controls. Figure Disclosures No relevant conflicts of interest to declare.

Download Full-text

Investigation of the effect of Prunus Amygdalus Amara on the expression of some genes of apoptosis and immortality in breast cancer cells (MCF-7)

Current Drug Research Reviews ◽

10.2174/2589977513666211202094433 ◽

2021 ◽

Vol 13 ◽

Author(s):

Maryam Abdolahi-Majd ◽

Gholamhossein Hassanshahi ◽

Mahboubeh Vatanparast ◽

Mojgan Noroozi Karimabad

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Pcr Analysis ◽

Mrna Levels ◽

Prunus Amygdalus ◽

Mcf7 Cells ◽

Significant Difference ◽

Anti Cancer ◽

Bitter Almond ◽

Mcf 7

Background: Anti-cancer effects of almond nuts or oil have been approved, but there are a few pieces of research that have evaluated, in detail, almond and other seeds' effects on cancer. Therefore, in the present project, the aim was to explore the regulatory effect of the bitter almond extract (Prunus amygdalus Batsch) on the apoptotic and anti-cancer potency of MCF-7 cells. Objectives: In the current experimental research, the Almond effect on MCF7 cells was evaluated by investigating the expression and the balance between Bcl-2, Bax genes to unmark the potential molecular mechanism. Methods: For 24 and 48h, the MCF7 cells were treated with the bitter almond extract (187.5-3000 µg/mL). MTT assay was used to assess the viability, and Real-time-PCR was applied to determine the expression of Bax and Bcl-2, facing β-actin. Results: Our results revealed a significant difference between different extract concentrations on the viability of MCF7 cell lines in 24 and 48 h; cell viability decreased time-dependently (P < 0.05). After 24 and 48h of extract facing MCF7 cells, the evaluated IC50 value was 3000 and 1500 µg/mL, respectively. Based on Real Time-PCR analysis, after 24 and 48 h, the mRNA levels of BCL-2 decreased by the extract, whereas BAX was in the MCF-7 cell line. Conclusion: From the results, it can be concluded that bitter almond extract has anti-cancer properties that may influence the apoptotic pathways by regulating relative gene expression.

Download Full-text

Abstract 1064: Pellino-1: A Novel Candidate In Vegf/Flk-1/MKK2 Signaling In Ischemic Preconditioning Induced Cardioprotection: A Study Using Flk +/− and MKK2 −/− Knockout Mice.

Circulation ◽

10.1161/circ.116.suppl_16.ii_213 ◽

2007 ◽

Vol 116 (suppl_16) ◽

Author(s):

Mahesh Thirunavukkarasu ◽

Samson Mathews Samuel ◽

Sankar Addya ◽

Lijun Zhan ◽

Chi-Kuang Huang ◽

...

Keyword(s):

Real Time ◽

Ischemic Preconditioning ◽

Knockout Mice ◽

Real Time Pcr ◽

Left Ventricular ◽

List Type ◽

Mrna Levels ◽

Clinical Issue ◽

Endothelial Cell Function ◽

Vegf Signaling

VEGF modulates the complex process of angiogenesis and other various aspects of endothelial cell function through either of its two tyrosine kinase receptors, VEGFR1/Flt-1 or VEGFR2/Flk1/ KDR via its target protein MKK2. In the present study we used Flk1 +/− and MKK2 −/− knockout mice in an attempt to address an important clinical issue by identifying potential downstream candidates of VEGF signaling through Flk1 receptor that trigger cardioprotective signal during ischemic preconditioning (IP). Mouse hearts were subjected to 30 min of global ischemia and 2 hours of reperfusion (IR) in the Isolated Working Heart model. It is known that IP (4min of ischemia + 6min reperfusion, 4 cycles, before 30 min of ischemia) induces cardioprotection through the activation of the VEGF signaling cascade. The mice were randomly divided into 6 groups for both the gene knockout (KO) studies: Wild Type-Baseline (WTBL), FlkBL/ MKK2BL (KOBL), WTIR , KOIR, WTIP and KOIP. Significant reduction in left ventricular functional recovery through out reperfusion (dp/dt = 605 vs 884), diminished coronary flow (1.9 vs 2.4) and aortic flow (0.16 vs 1.2) and increased infarct size (38.4% vs. 28.41%) after reperfusion were observed in FlkIR, compared to WTIR. As expected we observed disruption in IP induced cardioprotection in FlkIP compared to WTIP. Affymetrix gene chip analysis demonstrated significant downregulation of genes (Pellino-1, MKK2, NF-Î°B) which are thought to play important roles in cardioprotection after ischemic insults in the Flk +/− mice compared to WT. These results were further validated at the mRNA expression level with Real Time PCR. Pellino-1 (Pel-1) was found to be significantly downregulated in FlkBL (0.74 vs 1), FlkIR (1.29 vs 1.35) and FlkPC (1.35 vs 1.49) as compared to their respective controls. We further validated the mRNA levels of Pel-1using Real Time PCR and RT-PCR in the MKK2 −/− mice and found that it, remained unaffected in MKK2BL as compared to its WTBL, and increased as expected in MKK2PC as compared to both MKK2BL and FlkPC (2.48 vs 1.2 and 2.48 vs 1.35, respectively). Therefore this study validated for the first time that Pel-1 is a novel downstream mediator in VEGF/FLK1 signaling and it induces IP mediated cardioprotection via MKK2 signaling.

Download Full-text