Int J App Pharm, Vol 14, Issue 5, 2022, 32-40Review Article

NIOSOMES VERSUS PRONIOSOMES AS PROMISING DRUG DELIVERY SYSTEMS IN TREATMENT OF DIABETES MELLITUS

MAHMOUD H. TEAIMA¹, MOSTAFA I. GEBRIL², FATHY I. ABD ALLAH^3,4, MOHAMED A. EL-NABARAWI^1*

¹Department of Pharmaceutics and Industrial Pharmacy, Faculty of Pharmacy, Cairo University, Cairo, Egypt, ²Department of Pharmaceutics and Industrial Pharmacy, Faculty of Pharmacy, Badr University in Cairo (BUC), Badr City, Cairo, 11829, Egypt, ³International Center for Bioavailability, Pharmaceutical and Clinical Research, Obour City 11828, Egypt, ⁴Department of Pharmaceutics and Industrial Pharmacy, Faculty of Pharmacy, Al-Azhar University, Cairo 11651, Egypt
Email: mahmoud.teaima@pharma.cu.edu.eg

Received: 02 Jan 2022, Revised and Accepted: 30 Jul 2022

---

ABSTRACT

Diabetes Mellitus (DM) has emerged as an epidemic that has affected millions of people globally in the last few decades. Conventional antidiabetic dosage forms have a lot of problems that necessitate searching for novel drug delivery systems to overcome these drawbacks. Niosomes and proniosomes have been used to carry a wide variety of antidiabetic drugs achieving controlled and sustained release, which improves patient compliance. This review article describes the fundamental aspects of niosomes and proniosomes, including their structural components, methods of preparation, advantages and drawbacks, characterization, factors affecting niosomes formation along with their application in the treatment of diabetes. It also highlights the participation of other drug delivery systems in the treatment of diabetes done, mainly in the last decade.

Keywords: Diabetes mellitus (DM), Niosomes, Proniosomes, Ethosomes, Nanoparticles

---

© 2022 The Authors. Published by Innovare Academic Sciences Pvt Ltd. This is an open access article under the CC BY license (https://creativecommons.org/licenses/by/4.0/)
DOI: https://dx.doi.org/10.22159/ijap.2022v14i5.44039. Journal homepage: https://innovareacademics.in/journals/index.php/ijap

INTRODUCTION

Diabetes Mellitus (DM) is a multi-factorial chronic pathological condition of elevated blood glucose level (BGL) caused by multiple genetic and/or environmental factors, more specifically due to either deficiency of secretion of insulin hormone or due to pancreatic β cells destruction. It may also be caused by the non-utilization of insulin due to insulin resistance (IR) [1, 2]. Diabetes mellitus (DM) is a major health issue, its prevalence presents a real threat to humans [3]. The possibility of diabetes varies in different ethnicities, such as black and Hispanic people, and some minorities, like American Indians and Natives of Alaska, are more likely to have diabetes for a specific genetic profile. Though a lot of antidiabetic drugs are present in the market, achieving a complete and successful cure for DM remains a problem as there are a lot of adverse effects associated with these medications like gastric irritation, phobia of injection, transient nausea, diarrhea, loss of appetite and many more. Also, frequent daily administration of conventional antidiabetic drugs leads finally to patient incompliance [4, 5]. Nanotechnology showed a promising role in the management of diabetes mellitus in the last few years. Vesicular drug delivery systems have gained wide attention in the field of nanotechnology. These systems have the potential to carry a variety of drugs and have been widely used for various goals such as drug targeting, controlled and sustained release, and enhancement of permeation for drugs with low permeability [6]. Nanotechnological systems overcome conventional dosage forms drawbacks such as low aqueous solubility, poor bioavailability, low membrane permeability, variable plasma concentration, undesirable effects, and of course, poor patient compliance because of multiple administration [7, 8].

Nanotechnological systems such as liposomes and niosomes can carry both hydrophilic and hydrophobic drug moieties by encapsulation and partitioning into hydrophobic and hydrophilic parts also act as drug reservoirs [9].

A lot of advantages, but some physical and chemical problems made liposomes unsuitable for oral administration, such as hydrolysis and degradation of phospholipids or problems associated with storage for a long time as aggregation, fusion or leakage, and oxidation in aqueous systems [10]. These drawbacks of liposomes opens the door for niosomes to make remarkable progress.

From the last decade onwards, Niosomes and proniosomes are used to improve oral bioavailability of antidiabetic drugs. Searched keywords include niosomes, proniosomes and diabetes mellitus. Sources include recently published review articles and papers mainly published in the last ten years. This review attempts to provide all the basic details about niosomes and proniosomes that were published mainly in the last decade. It focuses mainly on preparation methods of both niosomes and proniosomes, factors affecting their formation, characterization, advantages, disadvantages, and their application in the treatment of diabetes as well as the new achievements in other drug delivery systems to improve the treatment of diabetes. The next trend is using other nano drug delivery systems to improve bioavailability of antidiabetic drugs much more.

Types of diabetes mellitus (DM)

It is important to determine the type of diabetes to choose the right therapy. American Diabetes Association (ADA) sets the following classification [11]:

• Type 1 diabetes mellitus (T1DM) occurs due to autoimmune β-cell destruction, usually leading to absolute insulin deficiency.

• Type 2 diabetes mellitus (T2DM) occurs due to a progressive loss of β-cell insulin secretion frequently on the background of insulin resistance.

• Gestational diabetes mellitus (GDM) is diagnosed in the second or third trimester of pregnancy that was not overt before gestation.

• Specific types of diabetes due to other causes e. g., monogenic diabetes syndromes (such as neonatal diabetes and maturity-onset diabetes of the young (MODY)), diseases of the exocrine pancreas (such as cystic fibrosis and pancreatitis), and drug or chemical-induced diabetes (such as with glucocorticoid use, in the treatment of HIV/AIDS, or after organ transplantation).

The two main types are (T1DM) and (T2DM) [12]:

Fig. 1: Comparison between type 1 and type 2 diabetes mellitus [12]

There are many types of anti-diabetic drugs that exert their hypoglycemic effects via different mechanisms. The four major groups of anti-diabetic agents are [1]:

• Biguanides act mainly by reducing gluconeogenesis in the liver. The most known example of biguanides is Metformin which is the first-line oral drug of choice in the management of T2DM across all age groups. Metformin activates adenosine monophosphate-activated protein kinase in the liver, causing glucose uptake by the liver and inhibiting gluconeogenesis through complex effects on the mitochondrial enzymes [13].

• Insulin secretagogues include both meglitinides group, like repaglinide, and the sulfonylureas group. Their mechanism of action is increasing plasma insulin concentrations. Consequently, they can be used only when residual pancreatic β-cells are present. They rise plasma insulin levels by two mechanisms: the first mechanism is the stimulation of insulin secretion by pancreatic β-cells, the second one is decreasing insulin clearance by the liver [14].

• Insulin sensitizers, like thiazolidinediones for example, pioglitazone and rosiglitazone, have proven to be effective in improving the sensitivity of peripheral tissues to insulin, and also effective in hyperglycemia and lipid metabolism [15].

• Insulin or its analogs provide exogenous insulin in the form of recombinant insulin.

Niosomes components

Non-ionic surfactants

The most widely used non-ionic surfactants as niosomal drug delivery carriers are alkyl ethers and alkyl esters due to their availability and low issues of toxicity. They include Alkyl ethers such as (Brij) and alkyl esters as sorbitan fatty acid esters (Span) and polyoxyethylene sorbitan fatty acid esters (Tween). Cell culture toxicity studies have shown that niosomes composed of ester-type surfactants are less toxic than ether-type ones. This could be attributed to the possible enzymatic degradation of ester bonds [16]. These surfactants have been used in manufacturing niosomes with various routes of administration including nasal [17], oral [18], transdermal [19, 20], and ocular delivery [21–23].

Cholesterol (bilayer membrane stabilizer)

Cholesterol forms hydrogen bonds with hydrophilic surfactant heads in the bilayer structure of niosomes [19, 53]. Therefore cholesterol content affects niosomes structure and physical properties such as entrapment efficiency (E. E %), long time stability [24, 25].

Charge inducers

Aggregation is one of the most frequent physical instabilities of niosomes followed by fusion. Electrostatic stabilization of the niosomes can strongly suppress their aggregation [26]. Incorporation of positive and negative charge inducers in the bilayer membranes, such as Stearyl amine and dicetyl phosphate, can improve the physical stability of the niosomes against aggregation [16].

Niosomes consist of a bi-layered structure of non-ionic surfactants (fig. 2). When surfactants and cholesterol are mixed in a proper ratio and the temperature is above the gel liquid transition temperature, These thermodynamically stable bilayered structures are formed [27]. Depending on their size, these second-generation elastic vesicles can be divided into three types (fig. 3), small unilamellar vesicles (SUV) (10–100 nm), large unilamellar vesicles (LUV) (100–3000 nm), and multi-lamellar vesicles (MLV) in which more than one bilayer is present [28].

Fig. 2: Structure of niosomes [29]

Fig. 3: Schematic structure of SUV, LUV, and MLV [30]

Advantages of niosomes

• Niosomes act as a reservoir to release the drug in a sustained pattern [31].

• They are biodegradable, biocompatible, and non-immunogenic, which made them an excellent choice [32].

• They can encapsulate large quantities of the drug in a relatively small volume of vesicles [33].

• Lipophilic drugs, hydrophilic drugs as well as amphiphilic drugs can be encapsulated in niosomes due to their unique structure [34, 35].

• Diverse administration routes (intravenous, oral, topical, etc.).

• In comparison with liposomes, Niosomes are more stable against chemical degradation or oxidation so they have a longer storage time [36].

Drawbacks of niosomes

• Physical instability problems such as aggregation, fusion, and leaking during storage and distribution, etc can be avoided by preparing proniosomes [37].

• The toxicity of the nonionic surfactants is not fully studied.

• Sterilization processes using heat, whether steam or dry heat sterilization, can cause bilayer destruction as the temperature exceeds the gel-liquid transition temperature of the surfactants, So the entrapped drug in the niosome bilayers leaked [38].

• Multilamellar vesicles preparation requires time and need specific tools [39].

Methods of preparation of niosomes

The widely reported preparation techniques are [40]:

Thin-film hydration (handshaking) technique

It is a simple technique; however, one of its disadvantages is that it involves the use of organic solvents to dissolve surfactants and cholesterol. In a round bottom flask surfactants and cholesterol are dissolved in chloroform or any suitable organic solvent followed by evaporation of that solvent to form a thin film on the bottom of the flask. That technique should be done at a temperature above the transition temperature of the surfactant. Hydration of this thin film produces multilamellar vesicles which are then sonicated to produce unilamellar vesicles [30, 41–44]. Niosomes prepared by this method have been reported to enhance the bioavailability of several anti-diabetic drugs, for example, repaglinide [45] and glimepiride [46].

Ether injection method

Both surfactant and drug are dissolved in diethyl ether and injected slowly through a needle with certain specifications to an aqueous phase, then heated above the boiling point of the organic solvent. This method produces large unilamellar vesicles (LUVs) and is further sonicated to obtain the required size [47–49].

Reverse phase evaporation method

Surfactants and cholesterol are dissolved in diethyl ether followed by the addition of the aqueous drug solution; then, the mixture was sonicated/homogenized. The organic layer was evaporated at room temperature under reduced pressure till niosomal suspension was formed [50, 51].

Trans-membrane pH gradient drug uptake process

In this method, both surfactant and cholesterol are dissolved in an organic solvent that is evaporated under reduced pressure, this leads to the formation of a thin film on the wall of the round bottom flask. This film is hydrated with citric acid and vortexed for a few minutes, so multilamellar vesicles (MLV) are formed. The resulting MLV are frozen and thawed thrice and then sonicated. Then aqueous phase is added and vortexed. The pH is adjusted finally to 7.0–7.2 by using disodium hydrogen phosphate. The resulting suspension is heated finally to 60 °C for 10 Min to obtain niosomes [26].

Emulsion method

Surfactants and cholesterol are dissolved in an organic solvent and then added to the drug previously dissolved in water. The formed emulsion is then heated to evaporate the organic solvent to obtain the niosomal formulation [52].

Bubble method

The most important advantage of this method is that it allows the preparation of niosomes without using organic solvents. In an aqueous phase, under a nitrogen atmosphere at 70 °C, Surfactants and additives are mixed. Mixing accomplished for 15s with high-speed homogenizer. In the last step, nitrogen bubbles are blown through the mixture at 70 °C to obtain niosomes as shown in fig. 4 [40, 53, 54].

Proniosome preparation

A lot of advantages are associated with this method, including rapid production process and ease of application. In this method, a water-soluble carrier is coated with a surfactant. Then the carrier is resolved during the hydration process at a temperature above the surfactant transition temperature, whereby niosomes are formed [55].

Fig. 4: Schematic diagram of bubble method [29]

Microfluidization method

This newly developed method produces smaller unilamellar vesicles with narrow size distribution. Across an interaction chamber, a solution of both drug and surfactants is pumped under a pressure rate of 100 ml/min [35]. This heat produced during microfluidization is removed by passing across a cooling loop to form niosomes [47].

Heating method

Both surfactant and cholesterol are hydrated separately in a buffer solution. After hydration, the cholesterol solution is heated for 1 h at 120 °C to be dissolved. Then the temperature of the solution is lowered, and surfactant and other additives are added to the buffer solution with continuous stirring. These formed niosomes are kept at room temperature for 30 min. Finally, niosomes are stored at 4–5 °C in a nitrogen atmosphere [24, 30, 56–58].

Proniosomes

Niosomal formulations show various advantages, such as improving the solubility and bioavailability of some poorly soluble drugs, as shown for acyclovir and griseofulvin, and maintaining good chemical stability during storage e. g. encapsulation increase the stability of peptide drugs [59]. Furthermore, low cost, more stability, ease of handling, formulation, and storage, less prone to oxidation make them a promising drug delivery system and superior to liposomes [13, 60]. On the other hand, Niosomes have some disadvantages which limit their shelf life, such as fusion, aggregation, sedimentation, leakage of entrapped drugs on storage, and loss of vesicular integrity [61–64].

To overcome all defects associated with niosomes, provesicular carrier systems are formulated i.e. anhydrous free-flowing proniosomal formulations. They can easily be reconstituted with the aqueous phase before administration or hydrated in body compartments to form niosomal vesicles (fig. 5) and these proniosomes-derived niosomes are more stable than conventional niosomes [65, 66].

Methods of preparation of proniosomes

There are different methods used for the preparation of proniosomes:

Fig. 5: Hydration of proniosomes into niosomes and hydrophilic and hydrophobic regions of niosomes [66]

Slurry method

This method includes Using carrier, surfactant, and organic solvent in a round bottom flask to obtain a slurry. The slurry is dried by applying vacuum to get free-flowing powder of proniosomes. The powder should be stored at 4 C in a sealed container [67].

Coacervation–phase separation technique

Previously determined amounts of both surface-active agent and cholesterol were mixed in glass vials. Small amount of absolute ethanol, typically half the weight of total lipids, enough to solubilize the lipids were added to the surfactant or surfactant/cholesterol mixture, and then, vials were tightly sealed and warmed in a water bath (55–60 °C) for 5 min while shaking until complete dissolution of lipids. To each of the formed transparent hot lipid solutions, an aqueous phase heated to 55–60 °C was added to the lipid solution while warming in the water bath for 3–5 min until a clear or translucent solution was produced. White creamy proniosomal gels were formed when the mixtures were allowed to cool down at room temperature [68].

Spray-coating method

This method involves the preparation of proniosomes by spraying surfactant/drug in an organic solvent onto a carrier or coating material and then evaporating the solvent [69].

Factors affecting niosomes formation

Type of surfactants used and charge inducers

Surfactants have a unique chemical structure which gives them dual properties. Nonionic surfactants are the main elements of niosomes. Various nonionic surfactants with different HLB values are used for the preparation of niosomes. The formation of niosomes and the encapsulation of drugs are influenced by the structure of surfactants. As the length of the alkyl chain of spans was increased, the entrapment efficiency of clarithromycin improved as reported by [70].

Addition of charge inducers

Adding some charge inducers such as dicetyl phosphate (negatively charged) and stearyl amine (positively charged) can stabilize niosomal formulations by imparting charge on niosomes surface, causing electrostatic repulsion, which prevents aggregation and coalescence [16, 30, 36, 39, 59].

Effect of encapsulated drug

An Important factor to be taken into consideration while formulating niosomes is the nature of the entrapped drug or in other words, the physicochemical characteristics of the drug. Drug characteristics such as molecular weight, structure, whether it is hydrophobic, hydrophilic, amphiphilic, etc. All of these factors have a great effect on both entrapment efficiency and the size of niosomes [71–73]. As reported in several articles, the maximum entrapment efficiency for a hydrophilic drug in niosomes could be between 10–20% [74, 75]. But in contrast, it was reported that entrapment efficiency of the hydrophilic drug (gallidermin, positive charge) in anionic niosomes could be up to 45% due to the interaction between niosomes negative charge and gallidermin positive charge [76].

Hydration medium

Hydration medium is one of the factors that greatly affects the properties of the prepared niosomes. Phosphate buffer is the most commonly used hydration medium. It can be used with various pH values according to the solubility of the entrapped drug [72, 77]. For example, zidovudine niosomes were prepared using phosphate buffer saline pH 7.4 [78]. Also, the temperature of the hydration medium is a critical factor as it affects both the size and shape of niosomes. It should be above gel to liquid phase transitional temperature [77, 79].

Hydration time

As said before, hydration medium influences the characteristics of the prepared niosomes. It was found that hydration time also affects the size and entrapment efficiency of niosomes. In a previously published article, results showed that short hydration time (15 min) resulted in vesicles (before the sonication step) with larger sizes and slightly less drug entrapment efficiency compared to niosomes subjected to a longer period of hydration (60 min) [80].

Characterization of proniosomes

Size and morphology

Scanning Electron Microscope and Transmission Electron Microscope can be used to determine surface characteristics, size, and shape of niosomes. Formed proniosomes were spread on a glass slide and the structure of proniosomes was observed [81].

Charge of vesicle and zeta potential

The zeta potential of vesicles can indicate the stability of niosomes [82]. In general, concerning stability against aggregation and fusion, charged niosomes are generally more stable than uncharged vesicles [40]. Also, negative zeta potential values ranging between −41.7 and −58.4 mV are sufficiently high for electrostatic stabilization. Both surfactant type or encapsulation efficiencies might affect the zeta potential values. The zetasizer is used to determine surface zeta potential [30].

Entrapment efficiency

Entrapment efficiency can be expressed as the amount of drug incorporated into the niosomes and is normally defined as the percentage of niosomes bound drug to the total amount of drug added. Determination of the E. E% generally requires centrifugation of the preparation to separate free drug from the niosomes [83]. Determination of both entrapped and unentrapped drug allows calculation of entrapment efficiency. The entrapment efficiency can be calculated using the following formula [30, 84]:

Stability study

Stability study discusses Storage feasibility of niosomal drug. One of the most important characteristics of a successful dosage form is the Stability of vesicles. There are a lot of factors that influence the Stability of niosomes such as nature of the entrapped drug, its concentration, type of surfactant used, and cholesterol amount. Stability studies investigate the percentage of drug leaching from niosomes during storage and while in general circulation. Using conditions that simulate both situations, this leaching can be evaluated by determining mean vesicle size, size distribution, and entrapment efficiency over several month periods. The stability of niosomes can also be assessed under conditions that accelerate photodegradation such as exposure to fluorescent light and UV irradiation as done for tretinoin niosomes [85]. It is important to provide chemical stability to both the surfactant and drug components so that the stabilization strategies must be optimized depending on the agent to be entrapped [30].

In vitro studies

Depending on the administration route, in vitro release can be determined by inserting the niosomal suspension in a dialysis membrane and immersing it into a buffer at a definite temperature, and determining the content of the drug crossed into the buffer [30].

Table 1: Application of niosomes in improving bioavailability of antidiabetic drugs

Drugs	Type of formulation	Model	Results	References
Nateglinide	Proniosomal gel	In vitro release and in vivo study	Administration of nateglinide niosomal proconcentrate resulted in a rapid reduction in blood glucose level	[86]
Glimepiride	Proniosomal Gel	In vitro and in vivo studies	Improved entrapment efficiency	[87]
Pioglitazone	Niosomes prepared using span 20 and cholesterol	In vitro and in vivo studies in albino Wister rats	Maintain the drug at the site of treatment for a prolonged time, capable of supplying constant drug concentration for a longer duration as they sustain drug release	[88]
Repaglinide	Niosomes using span 60 and cholesterol	In vivo using male Wister rats	Increased repaglinide bioavailability which decreases dosing frequency from BID to OD	[89]
Metformin hydrochloride	Niosomes	In vitro	Prolonged drug release	[90]
		In vivo	Improved anti-diabetic effect
Gliclazide	Niosomes	In vivo	Increased entrapement efficiency so that oral bioavailability was improved	[91]
Nateglinide	Proniosome powder	In vivo	Increased drug bioavailability	[92]
Glipizide and metformin hydrochloride Pioglitazone	Hydrogen bonded niosomes niosomes transgel	In vitro In vitro	Promising combinatorial sustained-release system Skin permeation increased	[93] [94]
		In vivo	Better bioavailability and antidiabetic activity
Metformin	Niosomes using Spans/Tweens/Brijs with Cholesterol and dicetyl phosphate (DCP)	In vitro release studies with USP dissolution apparatus.	More stable vesicles, higher entrapment, and delayed-release formulation using span 60 with a longer chain length	[41]
Glipizide	Pronisomes using Span 60, cholesterol and coating agent either maltodextrin or sorbitol or mannitol	In vitro release	Using maltodextrin as a coating agent provides Consistent and prolonged release formula.	[41)
Metformin	Niosomes	In vitro release	Factors that lead to the best formula include 100 molar concentration of cholesterol and surfactant, Presence of DCP, an equimolar ratio of span 60: cholesterol, and 15 ml of hydration medium.	[95]
Metformin	Niosomes using either Span 60 or Span 40 or Tween 80 and cholesterol.	In vivo	Better sustained anti-diabetic effect than oral doses given daily.	[96]
Gliclazide	Niosomes using span 60 and cholesterol	In vivo	Cholesterol: surfactant ratio of 4:7 was found to achieve maximum entrapment of the drug. Additionally, the formulation showed good oral bioavailability of 89% in vivo.	[97]
Metformin	Niosomes using Span 40/cholesterol dicetyl phosphate and Dioleoyl-3-trimethylammonium propane (DOTAP)	In vivo and in vitro	The niosomal formulation showed a sustained release pattern which provides greater control of the hyperglycemic condition.	[90]
Pioglitazone	Niosomes using Cholesterol and span 20	In vitro and in vivo studies	The prepared formulation maintained steady drug concentration (sustained effect) for a longer duration of time, thereby enhancing the therapeutic action.	[98]

Tissue distribution and in vivo studies

To know the distribution pattern of a certain drug, animals are sacrificed and various tissues such as kidney, liver, lungs, and heart are removed, washed with a buffer then homogenized and centrifuged, and after that, the supernatant is analyzed for the drug content [59]. Concerning niosomes In vivo studies, they depend on the route of administration, drug concentration, the effect of the drug, and the presence time of the drug in tissues such as the liver and lungs [27].

Application of niosomes

Niosomes can be used efficiently for enhancing the bioavailability of the entrapped drug; several studies showed an increase in the bioavailability of several drugs as shown in table 1.

Applications of other nanotechnological systems in the treatment of diabetes mellitus

There are a lot of novel drug delivery systems that were developed to overcome the drawbacks of niosomes and to attain maximum bioavailability of antidiabetics, as shown in table 2 below.

Table 2: Application of different drug delivery systems in enhancing the bioavailability of antidiabetic drugs

Drugs	Type of formulation	Model	Results	References
Repaglinide	Ethosomes	Ex-vivo drug permeation study and in vivo study	Repaglinide ethosomes showed a prolonged antidiabetic action suggesting a sustained release from the transdermal formulation.	[99]
Linagliptin	Solid lipid nanoparticles (SLNs)	Pharmacokinetic and pharmacodynamic study	SLNs showed improvement in linagliptin bioavailability which may be due to P-gp efflux inhibition and lymphatic targeting.	[100]
Glimepiride	Nanosuspension prepared by combination technique and precipitation technique	In vitro drug release	The formulation prepared by combination technique showed good solubility, dissolution, and drug release in comparison with the formulation prepared by nanoprecipitation technique.	[101]
Repaglinide	Nanoemulsion	In vivo study	Repaglinide nanoemulsion showed a better hypoglycemic effect than tablet formulation.	[102]
Glimepiride	Self nano-emulsifying system	Ex vivo skin permeation study and in vivo study	It enhanced Glimepiride skin permeability and significantly lowered and controlled the blood glucose level in diabetic rats.	[103]
Gliclazide	Nanocrystal	In vitro drug release and in vivo studies	The nanocrystal formulation provided initial faster release followed by delayed release, which facilitate delivery of gliclazide and maintained the glucose homeostasis in T2DM patients with better therapeutic activity.	[104]
Metformin	Carbon Nanotubes	In vivo study	Metformin-conjugated nanotubes maintained a reduced blood sugar level for a longer time than metformin alone	[105]
Liraglutide	Polymeric Nanoparticles using poly (lactic-co-glycolic acid) [PLGA]	In vitro release study, permeability study, and enzymatic degradation study	Polymeric nanoparticles protected liraglutide from degradation in the gastrointestinal tract, it also improved intestinal permeability, which enhanced oral bioavailability of the drug.	[106]
Glibenclamide	Polymeric Nanoparticles using hydroxypropyl methylcellulose (HPMC)	In vitro dissolution	Glibenclamide-loaded NPs showed higher drug dissolution (85%) in comparison with pure drug (35%) and commercial preparation (56%) in 5 min.	[107]

CONCLUSION

In recent years, niosomes and proniosomes have attracted great attention in the field of nanotechnology. This attention is increasing because of their ability to encapsulate both lipophilic and hydrophilic drugs. Niosomes achieved great advancement in treatment of diabetes through improving bioavailability of antidiabetic drugs with flexibility in route of administration. The future direction goes towards using other nanovesicles like ethosomes, cubosomes, transferosomes, Solid Lipid Nanoparticles (SLNs), Nanostructured Lipid Carriers (NLCs), and surface-modified niosomes to achieve drug targeting, which enhance the bioavailability of antidiabetic drugs with minimization of adverse effects. All of these vesicular drug delivery systems need further exploration to achieve the required outcome.

FUNDING

Nil

AUTHORS CONTRIBUTIONS

All authors have contributed equally.

CONFLICT OF INTERESTS

Declared none

REFERENCES

1. Artasensi A, Pedretti A, Vistoli G, Fumagalli L. Type 2 diabetes mellitus: a review of multi-target drugs. Molecules. 2020;25(8):1-20. doi: 10.3390/molecules25081987, PMID 32340373.

2. Matzinger M, Fischhuber K, Heiss EH. Activation of Nrf2 signaling by natural products-can it alleviate diabetes? Biotechnol Adv. 2018;36(6):1738-67. doi: 10.1016/ j.biotechadv.2017.12.015, PMID 29289692.

3. Khursheed R, Singh SK, Wadhwa S, Kapoor B, Gulati M, Kumar R. Treatment strategies against diabetes: success so far and challenges ahead. Eur J Pharmacol. 2019;862(Aug):172625. doi: 10.1016/j.ejphar.2019.172625. PMID 31449807.

4. Ensign LM, Cone R, Hanes J. Oral drug delivery with polymeric nanoparticles: the gastrointestinal mucus barriers. Adv Drug Deliv Rev. 2012;64(6):557-70. doi: 10.1016/j.addr. 2011.12.009. PMID 22212900.

5. Rai VK, Mishra N, Agrawal AK, Jain S, Yadav NP. Novel drug delivery system: an immense hope for diabetics. Drug Deliv. 2016;23(7):2371-90. doi: 10.3109/10717544.2014.991001, PMID 25544604.

6. Mir M, Ishtiaq S, Rabia S, Khatoon M, Zeb A, Khan GM. Nanotechnology: from in vivo imaging system to controlled drug delivery. Nanoscale Res Lett. 2017;12(1):500. doi: 10.1186/s11671-017-2249-8, PMID 28819800.

7. Bochot A, Fattal E. Liposomes for intravitreal drug delivery: A state of the art. J Control Release. 2012;161(2):628-34. doi: 10.1016/j.jconrel.2012.01.019, PMID 22289436.

8. Ahmad MZ, Akhter S, Mohsin N, Abdel-Wahab BA, Ahmad J, Warsi MH. Transformation of curcumin from food additive to multifunctional medicine: nanotechnology bridging the gap. Curr Drug Discov Technol. 2014;11(3):197-213. doi: 10.2174/1570163811666140616153436, PMID 24934264.

9. Kamel R, Basha M, Abd El-Alim SH. Development of a novel vesicular system using a binary mixture of sorbitan monostearate and polyethylene glycol fatty acid esters for rectal delivery of rutin. J Liposome Res. 2013;23(1):28-36. doi: 10.3109/08982104.2012.727422, PMID 23083098.

10. Khatoon M, Shah KU, Din FU, Shah SU, Rehman AU, Dilawar N. Proniosomes derived niosomes: recent advancements in drug delivery and targeting. Drug Deliv. 2017;24(Suppl1):56-69. doi: 10.1080/10717544.2017.1384520, PMID 29130758.

11. Care D, Suppl SS. Classification and diagnosis of diabetes: standards of medical care in diabetesd 2018. Diabetes Care. 2018;41(Jan):S13-27.

12. Zaric BL, Obradovic M, Sudar Milovanovic E, Nedeljkovic J, Lazic V, Isenovic ER. Drug delivery systems for diabetes treatment. Curr Pharm Des. 2019;25(2):166-73. doi: 10.2174/1381612825666190306153838, PMID 30848184.

13. Chaudhury A, Duvoor C, Reddy Dendi VS, Kraleti S, Chada A, Ravilla R. Clinical review of antidiabetic drugs: implications for type 2 diabetes mellitus management. Front Endocrinol (Lausanne). 2017;8(Jan):6. doi: 10.3389/fendo.2017.00006, PMID 28167928.

14. Sola D, Rossi L, Schianca GPC, Maffioli P, Bigliocca M, Mella R. Sulfonylureas and their use in clinical practice. Arch Med Sci. 2015;11(4):840-8. doi: 10.5114/aoms.2015.53304, PMID 26322096.

15. Davidson MA, Mattison DR, Azoulay L, Krewski D. Thiazolidinedione drugs in the treatment of type 2 diabetes mellitus: past, present and future. Crit Rev Toxicol. 2018;48(1):52-108. doi: 10.1080/10408444.2017.1351420, PMID 28816105.

16. Abdelkader H, Alani AWG, Alany RG. Recent advances in non-ionic surfactant vesicles (niosomes): self-assembly, fabrication, characterization, drug delivery applications and limitations. Drug Deliv. 2014;21(2):87-100. doi: 10.3109/10717544.2013.838077, PMID 24156390.

17. Ammar HO, Haider M, Ibrahim M, El Hoffy NM. In vitro and in vivo investigation for optimization of niosomal ability for sustainment and bioavailability enhancement of diltiazem after nasal administration. Drug Deliv. 2017;24(1):414-21. doi: 10.1080/10717544.2016.1259371, PMID 28165822.

18. Arafa MG, Ghalwash D, El-kersh DM, Elmazar MM. Propolis-based niosomes as oromuco-adhesive films: A randomized clinical trial of a therapeutic drug delivery platform for the treatment of oral recurrent aphthous ulcers. Sci Rep. 2018;8(1 Nov). doi: 10.1038/s41598-018-37157-7, PMID 30575794.

19. Salem HF, Kharshoum RM, Abou-Taleb HA, Farouk HO, Zaki RM. Fabrication and appraisal of simvastatin via tailored niosomal nanovesicles for transdermal delivery enhancement: in vitro and in vivo assessment. Pharmaceutics. 2021;13(2):1-25. doi: 10.3390/pharmaceutics13020138, PMID 33494472.

20. Auda SH, Fathalla D, Fetih G, El-Badry M, Shakeel F. Niosomes as transdermal drug delivery system for celecoxib: in vitro and in vivo studies. Polym Bull. 2016;73(5):1229-45. doi: 10.1007/s00289-015-1544-8.

21. Fathalla D, Fouad EA, Soliman GM. Latanoprost niosomes as a sustained release ocular delivery system for the management of glaucoma. Drug Dev Ind Pharm. 2020;46(5):806-13. doi: 10.1080/03639045.2020.1755305, PMID 32281424.

22. Abdelbary GA, Amin MM, Zakaria MY. Ocular ketoconazole-loaded proniosomal gels: formulation, ex vivo corneal permeation and in vivo studies. Drug Deliv. 2017;24(1):309-19. doi: 10.1080/10717544.2016.1247928, PMID 28165809.

23. Emad Eldeeb A, Salah S, Ghorab M. Proniosomal gel-derived niosomes: an approach to sustain and improve the ocular delivery of brimonidine tartrate; formulation, in vitro characterization, and in vivo pharmacodynamic study. Drug Deliv. 2019;26(1):509-21. doi: 10.1080/10717544. 2019.1609622, PMID 31090464.

24. Ag Seleci DA, Seleci M, Walter J, Stahl F, Scheper T. Niosomes as nanoparticular drug carriers: fundamentals and recent applications. Journal of Nanomaterials. 2016;2016(fig. 1). doi: 10.1155/2016/7372306.

25. Aher P, Dandgavhal K, Bhandari D, Saindane H, Deore N, Amrutkar S. Niosomes as a potential drug delivery system. IJPSRR. 2021;68(1):21-7. doi: 10.47583/ ijpsrr.2021.v68i01.004.

26. Azeem A, Anwer MK, Talegaonkar S. Niosomes in sustained and targeted drug delivery: some recent advances. J Drug Target. 2009;17(9):671-89. doi: 10.3109/10611860903079454, PMID 19845484.

27. Bhardwaj P, Tripathi P, Gupta R, Pandey S. Niosomes: a review on niosomal research in the last decade. J Drug Deliv Sci Technol. 2020;56(Jan):101581. doi: 10.1016/j.jddst.2020.101581.

28. Zhou X, Hao Y, Yuan L, Pradhan S, Shrestha K, Pradhan O. Nano-formulations for transdermal drug delivery: a review. Chin Chem Lett. 2018;29(12):1713-24. doi: 10.1016/j.cclet.2018.10.037.

29. Yeo PL, Lim CL, Chye SM, Kiong Ling APK, Koh RY. Niosomes: a review of their structure, properties, methods of preparation, and medical applications. Asian Biomed. 2018;11(4):301-14. doi: 10.1515/abm-2018-0002.

30. Moghassemi S, Hadjizadeh A. Nano-niosomes as nanoscale drug delivery systems: an illustrated review. J Control Release. 2014;185(1):22-36. doi: 10.1016/j.jconrel.2014.04.015, PMID 24747765.

31. Khoee S, Yaghoobian M. Niosomes: a novel approach in modern drug delivery systems. Elsevier Inc; 2017. p. 207-37. doi: 10.1016/B978-0-323-46143-6/00006-3.

32. Waddad AY, Abbad S, Yu F, Munyendo WLL, Wang J, Lv H. Formulation, characterization and pharmacokinetics of Morin hydrate niosomes prepared from various non-ionic surfactants. Int J Pharm. 2013;456(2):446-58. doi: 10.1016/j.ijpharm.2013.08.040, PMID 23998955.

33. Nasr M, Mansour S, Mortada ND, Elshamy AA. Vesicular aceclofenac systems: A comparative study between liposomes and niosomes. J Microencapsul. 2008;25(7):499-512. doi: 10.1080/02652040802055411, PMID 18608811.

34. Master AM, Rodriguez ME, Kenney ME, Oleinick NL, Gupta AS. Delivery of the photosensitizer Pc 4 in PEG–PCL micelles for in vitro PDT studies. J Pharm Sci. 2010;99(5):2386-98. doi: 10.1002/jps.22007, PMID 19967780://www.ncbi.nlm.nih.gov/ pubmed/19967780.

35. Saraswathi TS, Mothilal M, Jaganathan MK. Niosomes as an emerging formulation tool for drug delivery-a review. Int J Appl Pharm. 2019;11(2):7-15.

36. Uchegbu IF, Vyas SP. Non-ionic surfactant-based vesicles (niosomes) in drug delivery. International Journal of Pharmaceutics. 1998;172(1-2):33-70. doi: 10.1016/S0378-5173(98)00169-0.

37. Ammar HO, Ghorab M, El-Nahhas SA, Higazy IM. Proniosomes as a carrier system for transdermal delivery of tenoxicam. Int J Pharm. 2011;405(1-2):142-52. doi: 10.1016/j.ijpharm.2010.11.003. PMID 21129461.

38. Masjedi M, Montahaei T. An illustrated review on nonionic surfactant vesicles (niosomes) as an approach in modern drug delivery: fabrication, characterization, pharmaceutical, and cosmetic applications. J Drug Deliv Sci Technol. 2021;61. doi: 10.1016/j.jddst.2020.102234.

39. Gharbavi M, Amani J, Kheiri Manjili H, Danafar H, Sharafi A. Niosome: A promising nanocarrier for natural drug delivery through the blood-brain barrier. Adv Pharmacol Sci. 2018;2018:6847971. doi: 10.1155/2018/6847971, PMID 30651728.

40. Amoabediny G, Haghiralsadat F, Naderinezhad S, Helder MN, Akhoundi Kharanaghi E, Mohammadnejad Arough J. Overview of preparation methods of polymeric and lipid-based (niosome, solid lipid, liposome) nanoparticles: A comprehensive review. Int J Polym Mater Polym Biomater. 2018;67(6):383-400. doi: 10.1080/00914037.2017.1332623.

41. Marianecci C, Di Marzio L, Rinaldi F, Celia C, Paolino D, Alhaique F. Niosomes from 80s to present: the state of the art. Adv Colloid Interface Sci. 2014;205:187-206. doi: 10.1016/j.cis.2013.11.018. PMID 24369107.

42. Manconi M, Sinico C, Valenti D, Loy G, Fadda AM. Niosomes as carriers for tretinoin. I. Preparation and properties. Int J Pharm. 2002;234(1-2):237-48. doi: 10.1016/s0378-5173(01)00971-1, PMID 11839454.

43. Uchegbu IF, Duncan R. Niosomes containing N-(2-hydroxypropyl)methacrylamide copolymer-doxorubicin (PK1): effect of method of preparation and choice of surfactant on niosome characteristics and a preliminary study of body distribution. International Journal of Pharmaceutics. 1997;155(1):7-17. doi: 10.1016/S0378-5173(97)00141-5.

44. Thabet Y, Elsabahy M, Eissa NG. Methods for preparation of niosomes: A focus on thin-film hydration method. Methods. 2022;199:9-15. doi: 10.1016/j.ymeth.2021.05.004. PMID 34000392.

45. Yaghoobian M, Haeri A, Bolourchian N, Shahhosseni S, Dadashzadeh S. The impact of surfactant composition and surface charge of niosomes on the oral absorption of repaglinide as a BCS II model drug. Int J Nanomedicine. 2020;15:8767-81. doi: 10.2147/IJN.S261932, PMID 33204087.

46. Mohsen AM, AbouSamra MM, ElShebiney SA. Enhanced oral bioavailability and sustained delivery of glimepiride via niosomal encapsulation: in vitro characterization and in vivo evaluation. Drug Dev Ind Pharm. 2017;43(8):1254-64. doi: 10.1080/03639045.2017.1310224, PMID 28330377.

47. Chen S, Hanning S, Falconer J, Locke M, Wen J. Recent advances in non-ionic surfactant vesicles (niosomes): fabrication, characterization, pharmaceutical and cosmetic applications. Eur J Pharm Biopharm. 2019;144(Aug):18-39. doi: 10.1016/j.ejpb.2019.08.015, PMID 31446046.

48. Patel P, Barot T, Kulkarni P. Formulation, Characterization and in vitro and in vivo evaluation of capecitabine loaded niosomes. Curr Drug Deliv. 2020;17(3):257-68. doi: 10.2174/1567201817666200214111815, PMID 32056523.

49. A RZM, B KD, C RBB. Niosomal drug delivery SYSTEM–a review academic sciences; 2011.

50. Bendas ER, Abdullah H, El-Komy MHM, Kassem MAA. Hydroxychloroquine niosomes: A new trend in topical management of oral lichen planus. Int J Pharm. 2013;458(2):287-95. doi: 10.1016/j.ijpharm.2013.10.042, PMID 24184035.

51. Kusuma Priya MD, Kumar V, Damini VK, Eswar K, Reddy KR, Brito Raj S. Somes: a review on composition, formulation methods and evaluations of different types of ’somes’ drug delivery system. Int J Appl Pharm. 2020;12(6):7-18.

52. Bhattacharya S, Kumar N, Singhai M, Setia A, Chaudhary A, Sagar S. Preparation and evaluation of diclofenac sodium niosomes using round bottom flask method. Asian J Pharm. 2020;14(2):188-94.

53. Talsma H, Van Steenbergen MJ, Borchert JCH, Crommelin DJA. A novel technique for the one‐step preparation of liposomes and nonionic surfactant vesicles without the use of organic solvents. Liposome formation in a continuous gas stream: the ’Bubble’ method. J Pharm Sci. 1994;83(3):276-80. doi: 10.1002/jps.2600830303, PMID 8207668.

54. More VV, Gilhotra RM, Nitalikar MM, Khule PK. Niosomal drug delivery-A comprehensive review. Asian J Pharm. 2018 Oct 1;12:S1159-64.

55. Sankar V, Ruckmani K, Durga S, Jailani S. Proniosomes as drug carriers. Pak J Pharm Sci. 2010;23(1):103-7. PMID 20067875.

56. Mozafari MR. A new technique for the preparation of nontoxic liposomes and nanoliposomes: the heating method. Nanoliposomes Fundam Recent Dev. 2005:91-8.

57. Mozafari MR, Reed CJ, Rostron C. Cytotoxicity evaluation of anionic nanoliposomes and nanolipoplexes prepared by the heating method without employing volatile solvents and detergents. Pharmazie. 2007;62(3):205-9. PMID 17416197.

58. Mozafari MR, Reed CJ, Rostron C, Kocum C, Piskin E. Construction of stable anionic liposome-plasmid particles using the heating method: A preliminary investigation. Cell Mol Biol Lett. 2002;7(3):923-7. PMID 12378277.

59. Rajera R, Nagpal K, Singh SK, Mishra DN. Niosomes: A controlled and novel drug delivery system. Biol Pharm Bull. 2011;34(7):945-53. doi: 10.1248/bpb.34.945, PMID 21719996.

60. Paecharoenchai O, Teng L, Yung BC, Teng L, Opanasopit P, Lee RJ. Nonionic surfactant vesicles for delivery of RNAi therapeutics. Nanomedicine (Lond). 2013;8(11):1865-73. doi: 10.2217/nnm.13.155, PMID 24156490.

61. El-Laithy HM, Shoukry O, Mahran LG. Novel sugar esters proniosomes for transdermal delivery of vinpocetine: preclinical and clinical studies. Eur J Pharm Biopharm. 2011;77(1):43-55. doi: 10.1016/j.ejpb.2010.10.011, PMID 21056658.

62. El Maghraby GM, Ahmed AA, Osman MA. Penetration enhancers in proteasomes as a new strategy for enhanced transdermal drug delivery. Saudi Pharm J. 2015;23(1):67-74. doi: 10.1016/j.jsps.2014.05.001. PMID 25685045.

63. Madan JR, Ghuge NP, Dua K. Formulation and evaluation of proniosomes containing lornoxicam. Drug Deliv Transl Res. 2016;6(5):511-8. doi: 10.1007/s13346-016-0296-9, PMID 27255375.

64. Shaker DS. Bioavailability and hypocholesterolemic effect of proniosomal simvastatin for transdermal delivery. Int J Pharm Pharm Sci. 2013;5(4):344-51.

65. Rahman SA, Abdelmalak NS, Badawi A, Elbayoumy T, Sabry N, El Ramly A. Formulation of tretinoin-loaded topical proniosomes for treatment of acne: in vitro characterization, skin irritation test and comparative clinical study. Drug Deliv. 2015;22(6):731-9. doi: 10.3109/10717544.2014.896428, PMID 24670094.

66. Ge X, Wei M, He S, Yuan WE. Advances of non-ionic surfactant vesicles (niosomes) and their application in drug delivery. Pharmaceutics. 2019;11(2). doi: 10.3390/pharmaceutics11020055, PMID 30700021.

67. Yasam VR, Jakki SL, Natarajan J, Kuppusamy G. A review on novel vesicular drug delivery: proniosomes. Drug Deliv. 2014;21(4):243-9. doi: 10.3109/10717544.2013.841783, PMID 24128089.

68. Vora B, Khopade AJ, Jain NK. Proniosome-based transdermal delivery of levonorgestrel for effective contraception. J Control Release. 1998;54(2):149-65. doi: 10.1016/s0168-3659(97)00100-4, PMID 9724902.

69. Ahmad MZ, Mohammed AA, Mokhtar Ibrahim M. Technology overview and drug delivery application of proniosome. Pharm Dev Technol. 2017;22(3):302-11. doi: 10.3109/10837450.2015.1135344, PMID 26794727.

70. Shilakari Asthana GS, Sharma PK, Asthana A. In vitro and in vivo evaluation of niosomal formulation for controlled delivery of clarithromycin. Scientifica (Cairo). 2016;2016:6492953. doi: 10.1155/2016/6492953, PMID 27293976.

71. G DB, P VL. Recent advances of nonionic surfactant-based nanovesicles (niosomes and proniosomes): a brief review of these in enhancing transdermal delivery of drug. Futur J Pharm Sci. 2020;6(1).

72. Kumar GP, Rajeshwarrao P. Nonionic surfactant vesicular systems for effective drug delivery-an overview. Acta Pharmaceutica Sinica B. 2011;1(4):208-19. doi: 10.1016/j.apsb.2011.09.002.

73. A RZM, B RBB. Niosomes-challenge in preparation for pharmaceutical scientist Academic Sciences; 2014.

74. Iii III. Current techniques series; 1984. p. 258-60.

75. Peltonen L, Koistinen P, Karjalainen M, Häkkinen A, Hirvonen J. The effect of cosolvents on the formulation of nanoparticles from low-molecular-weight poly(l)lactide. AAPS PharmSciTech. 2002;3(4):1–7E32. doi: 10.1208/pt030432, PMID 12916926.

76. Manosroi A, Khanrin P, Lohcharoenkal W, Werner RG, Gotz F, Manosroi W. Transdermal absorption enhancement through rat skin of gallidermin loaded in niosomes. Int J Pharm. 2010;392(1-2):304-10. doi: 10.1016/j.ijpharm.2010.03.064, PMID 20381599.

77. Mahale NB, Thakkar PD, Mali RG, Walunj DR, Chaudhari SR. Niosomes: novel sustained release nonionic stable vesicular systems-an overview. Adv Colloid Interface Sci. 2012;183-184:46-54. doi: 10.1016/j.cis.2012.08.002. PMID 22947187.

78. Ruckmani K, Sankar V. Formulation and optimization of zidovudine niosomes. AAPS PharmSciTech. 2010;11(3):1119-27. doi: 10.1208/s12249-010-9480-2, PMID 20635228.

79. Nasseri B. Effect of cholesterol and temperature on the elastic properties of niosomal membranes. Int J Pharm. 2005;300(1-2):95-101. doi: 10.1016/j.ijpharm.2005.05.009, PMID 16006080.

80. Yeo LK, Chaw CS, Elkordy AA. The effects of hydration parameters and co-surfactants on methylene blue-loaded niosomes prepared by the thin film hydration method. Pharmaceuticals (Basel). 2019;12(2). doi: 10.3390/ph12020046, PMID 30934834.

81. Ramkanth S, Chetty CM, Sudhakar Y, Thiruvengadarajan VS, Anitha P, Gopinath C. Development, characterization and in vivo evaluation of proniosomal based transdermal delivery system of Atenolol. Future Journal of Pharmaceutical Sciences. 2018;4(1):80-7. doi: 10.1016/j.fjps.2017.10.003.

82. Nasr A, Qushawy M, Swidan S. Spray dried lactose based proniosomes as stable provesicular drug delivery carriers: screening, formulation, and physicochemical characterization. Int J App Pharm. 2018;10(5):125-37. doi: 10.22159/ijap.2018v10i5.27732.

83. Kaoud RM, Heikal EJ, Hammady TM. Diacerein-loaded niosomes (Dc-Ns): a new technique to sustain the release of drug action. Int J App Pharm. 2022;14(1):156-63. doi: 10.22159/ijap.2022v14i1.43353.

84. Jadhav A, Varghese Cheriyan BV. Formulation and optimization of nifedipine-loaded nanocarriers. Int J App Pharm. 2021;13(5):311-7. doi: 10.22159/ijap.2021v13i5.42050.

85. Manconi M, Valenti D, Sinico C, Lai F, Loy G, Fadda AM. Niosomes as carriers for tretinoin. II. Influence of vesicular incorporation on tretinoin photostability. Int J Pharm. 2003;260(2):261-72. doi: 10.1016/s0378-5173(03)00268-0, PMID 12842345.

86. Sultan AA, El-Gizawy SA, Osman MA, El Maghraby GM. Niosomes for oral delivery of nateglinide: in situ–in vivo correlation. Journal of Liposome Research. Taylor and Francis. 2018;28(3):209-17. doi: 10.1080/08982104.2017.1343835, PMID 28618876.

87. Abdallah MH, Sabry SA, Hasan AA. Enhancing transdermal delivery of glimepiride via entrapment in proniosomal gel. J Young Pharm. 2016;8(4):335-40. doi: 10.5530/jyp.2016.4.8.

88. Haider MF, Kanoujia J, Tripathi CB, Arya M, Kaithwas G, Saraf SA. Pioglitazone loaded vesicular carriers for anti-diabetic activity: development and optimization as per central composite design. J Pharmaceut Sci Pharmacol. 2015 Mar 1;2(1):11-20. doi: 10.1166/jpsp.2015.1042.

89. Namdev S, Gujar K, Mandlik S, Jamkar P. Preparation and in vivo characterization of niosomal carriers of the antidiabetic drug repaglinide. PCI- Approved-IJPSN. 2015 Feb 28;8(1):2756-67. doi: 10.37285/ijpsn.2015.8.1.8/index.php/ijpsn/article/view/764.

90. Hasan AA, Madkor H, Wageh S. Formulation and evaluation of metformin hydrochloride-loaded niosomes as controlled release drug delivery system. Drug Deliv. 2013;20(3-4):120-6. doi: 10.3109/10717544.2013.779332, PMID 23651102.

91. Kesharwani P, Gorain B, Low SY, Tan SA, Ling ECS, Lim YK. Nanotechnology-based approaches for anti-diabetic drugs delivery. Diabetes Res Clin Pract. 2018;136:52-77. doi: 10.1016/j.diabres.2017.11.018, PMID 29196152.

92. Sahoo RK, Biswas N, Guha A, Kuotsu K. Maltodextrin based proniosomes of nateglinide: bioavailability assessment. Int J Biol Macromol. 2014;69:430-4. doi: 10.1016/ j.ijbiomac.2014.05.075, PMID 24909314.

93. Samed N, Sharma V, Sundaramurthy A. Hydrogen bonded niosomes for encapsulation and release of hydrophilic and hydrophobic anti-diabetic drugs: an efficient system for oral anti-diabetic formulation. Appl Surf Sci. 2018;449:567-73. doi: 10.1016/j.apsusc.2017.11.055.

94. Prasad PS, Imam SS, Aqil M, Sultana Y, Ali A. QbD-based carbopol transgel formulation: characterization, pharmacokinetic assessment and therapeutic efficacy in diabetes. Drug Deliv. 2016;23(3):1057-66. doi: 10.3109/10717544.2014.936536, PMID 25033041.

95. Sankhyan A, Pawar PK. Metformin loaded non-ionic surfactant vesicles: Optimization of formulation, effect of process variables and characterization. Daru J Pharm Sci Aru. 2013;21(1):1-8. doi: 10.1186/2008-2231-21-7, PMID 23351604.

96. El-Ridy MS, Yehia SA, Elsayed I, Younis MM, Abdel-Rahman RF, El-Gamil MA. Metformin hydrochloride and wound healing: from nanoformulation to pharmacological evaluation. J Liposome Res. 2019;29(4):343-56. doi: 10.1080/08982104.2018.1556291. PMID 30526146.

97. Rathi J, Tamizharasi S, Dubey A, Rathi V. Development and characterization of niosomal drug delivery of gliclazide. J Young Pharm Acists. 2009;1(3):205. doi: 10.4103/0975-1483.57065.

98. Haider MF, Kanoujia J, Tripathi CB, Arya M, Kaithwas G, Saraf SA. Pioglitazone loaded vesicular carriers for anti-diabetic activity: development and optimization as per central composite design. J Pharmaceut Sci Pharmacol. 2015;2(1):11-20. doi: 10.1166/jpsp.2015.1042.

99. Bodade SS, Shaikh KS, Kamble MS, Chaudhari PD. A study on ethosomes as mode for transdermal delivery of an antidiabetic drug. Drug Deliv. 2013;20(1):40-6. doi: 10.3109/10717544.2012.752420, PMID 23311652.

100. Shah P, Chavda K, Vyas B, Patel S. Formulation development of linagliptin solid lipid nanoparticles for oral bioavailability enhancement: role of P-gp inhibition. Drug Deliv Transl Res. 2021;11(3):1166-85. doi: 10.1007/s13346-020-00839-9, PMID 32804301.

101. Bose S, Sharma P, Mishra V, Patial S, Saraogi GK, Tambuwala MM. Comparative in vitro evaluation of glimepiride containing nanosuspension drug delivery system developed by different techniques. J Mol Struct. 2021;1231. doi: 10.1016/j.molstruc.2021.129927.

102. Akhtar J, Siddiqui HH, Fareed S, Badruddeen, Khalid KM, Aqil Khalid M, Aqil M. Nanoemulsion: for improved oral delivery of repaglinide. Drug Deliv. 2016;23(6):2026-34. doi: 10.3109/10717544.2015.1077290, PMID 27187792.

103. Ahmed OAA, Afouna MI, El-Say KM, Abdel-Naim AB, Khedr A, Banjar ZM. Optimization of self-nano emulsifying systems for the enhancement of in vivo hypoglycemic efficacy of glimepiride transdermal patches. Expert Opin Drug Deliv. 2014;11(7):1005-13. doi: 10.1517/17425247.2014.906402, PMID 24702435.

104. Panda BP, Krishnamoorthy R, Bhattamisra SK, Shivashekaregowda NKH, Seng LB, Patnaik S. Fabrication of second generation smarter PLGA based nanocrystal carriers for improvement of drug delivery and therapeutic efficacy of gliclazide in Type-2 diabetes rat model. Sci Rep. 2019;9(1):1–15. doi: 10.1038/s41598-019-53996-4, PMID 31758056.

105. Mirazi N, Shoaei J, Khazaei A, Hosseini A. A comparative study on effect of metformin and metformin-conjugated nanotubes on blood glucose homeostasis in diabetic rats. Eur J Drug Metab Pharmacokinet. 2015;40(3):343-8. doi: 10.1007/s13318-014-0213-x, PMID 24969688.

106. Ismail R, Bocsik A, Katona G, Grof I, Deli MA, Csoka I. Encapsulation in polymeric nanoparticles enhances the enzymatic stability and the permeability of the glpGLP-1 analog, liraglutide, across a culture model of intestinal permeability. Pharmaceutics. 2019;11(11):1-13. doi: 10.3390/pharmaceutics11110599, PMID 31726699.

107. Yu L, Li C, Le Y, Chen JF, Zou H. Stabilized amorphous glibenclamide nanoparticles by high-gravity technique. Mater Chem Phys. 2011;130(1-2):361-6, doi: 10.1016/ j.matchemphys.2011.06.049.